Beneficial microbes for delivery of effector peptides or proteins and use thereof

ABSTRACT

Disclosed are recombinant host cells comprising a promoter-effective nucleic acid molecule operably coupled to a nucleic acid molecule that encodes a plant effector protein or polypeptide that induces an active plant response including, among others, growth enhancement, disease resistance, pest or insect resistance, and stress resistance. Use of these recombinant host cells for modulating plant biochemical signaling, imparting disease resistance to plants, enhancing plant growth, imparting tolerance to biotic stress, imparting tolerance and resistance to abiotic stress, imparting desiccation resistance to cuttings removed from ornamental plants, imparting post-harvest disease or post-harvest desiccation resistance to a fruit or vegetable, or enhancing the longevity of fruit or vegetable ripeness are also disclosed.

This application is a divisional of U.S. patent application Ser. No. 15/476,257, filed Mar. 31, 2017, which claims the priority benefit of U.S. Provisional Patent Application Ser. No. 62/319,150, filed Apr. 6, 2016, which is hereby incorporated by reference in its entirety.

FIELD OF THE INVENTION

The present invention relates to recombinant beneficial microbes for delivery of plant effector proteins or polypeptides and their use for inducing active plant responses including, among others, growth enhancement, disease resistance, pest or insect resistance, and stress resistance.

BACKGROUND OF THE INVENTION

The identification and isolation of harpin proteins came from basic research at Cornell University attempting to understand how plant pathogenic bacteria interact with plants. A first line of defense is the hypersensitive response (HR), a localized plant cell death at the site of infection. Cell death creates a physical barrier to movement of the pathogen and in some plants dead cells can release compounds toxic to the invading pathogen. Research had indicated that pathogenic bacteria were likely to have a single factor that was responsible for triggering the HR. A basic aim of the Cornell research was to identify a specific bacterial protein responsible for eliciting the HR. The target protein was known to be encoded by one of a group of bacteria genes called the Hypersensitive Response and Pathogenicity (hrp) gene cluster. The hrp cluster in the bacterium Erwinia amylovora (Ea), which causes fire blight in pear and apple, was dissected and a single protein was identified that elicited HR in certain plants. This protein was given the name harpin (and, later, harpin_(Ea)) and the corresponding gene designated hrpN. This was the first example of such a protein and gene identified from any bacterial species.

A number of different harpin proteins have since been identified from Erwinia, Pseudomonas, Ralstonia, Xanthomonas, and Pantoea species, among others. Harpin proteins, while diverse at the primary amino acid sequence level, share common biochemical and biophysical characteristics as well as biological functions. Based on their unique properties, the harpin proteins are regarded in the literature as belonging to a single class of proteins.

Subsequent to their identification and isolation, it was thereafter discovered that harpins could elicit disease resistance in plants and increase plant growth. An important early finding was that application of purified harpin protein made a plant resistant to a subsequent pathogen attack, and in locations on the plant well away from the injection site. This meant that harpin proteins can trigger a Systemic Acquired Resistance (SAR), a plant defense mechanism that provides resistance to a variety of viral, bacterial, and fungal pathogens.

In crop protection, there is a continuous need for compositions that improve the health of plants. Healthier plants are desirable since they result in better yields and/or a better quality of the plants or crops. Healthier plants also better resist biotic and abiotic stress. A high resistance against biotic stresses in turn allows the growers to reduce the quantity of pesticides applied and consequently to slow down the development of resistances against the respective pesticides.

Harpin_(αβ) is a fusion protein that is derived from several different harpins. Harpin_(αβ) has been shown to suppress nematode egg production, enhance the growth, quality and yield of a plant, and increase a plant's vigor. Its amino acid and nucleotide sequences are described in detail in U.S. Application Publ. No. 2010/0043095.

To date, harpin and harpin_(αβ) production and their use in agricultural and horticultural applications have been as a powdered solid coated on starch. This limits the use and versatility of the harpin proteins, because liquid suspensions of the powdered harpin proteins in water have an effective useful life of only 48-72 hours before significant degradation and loss of activity occurs. Another problem with harpin solutions is protein solubility and stability.

Once solutions of the harpin proteins or polypeptides are applied topically to plants, the proteins or polypeptides will induce an active plant response, but the response typically is of a limited duration insofar as multiple applications are used over the course of a growing season. Indeed, the commercial instructions for using harpin_(αβ)-containing products recommend using liquid formulations within a short period of time (e.g., 8 or 24 hours) of mixing and, depending on the type of crop and benefits sought, multiple applications are often recommended. It would be desirable, therefore, to identify a mechanism for delivery of protein-based elicitor peptides that can be effective for prolonged period of time during the growing season so as to minimize the number of applications while also enhancing efficacy thereof.

The present invention is directed to overcoming these and other deficiencies in the art.

SUMMARY OF THE INVENTION

A first aspect of the invention relates to a recombinant host cell comprising a transgene that comprises a promoter-effective nucleic acid molecule operably coupled to a nucleic acid molecule that encodes a plant effector protein or polypeptide, wherein the recombinant host cell is a microbe that imparts a first benefit to a plant grown in the presence of the recombinant microbe and the plant effector protein or polypeptide imparts a second benefit to the plant grown in the presence of the recombinant microbe.

A second aspect of the invention relates to a composition that includes a plurality of recombinant host cells according to the first aspect of the invention.

A third aspect of the invention relates to a method for treating plant seeds. This method includes: providing one or more plant seeds and applying to the provided one or more plant seeds either a recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention.

A fourth aspect of the invention relates to a method for treating plants. This method includes: providing one or more plants and applying to the provided one or more plants either a recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention.

A fifth aspect of the invention relates to a method for treating plants. This method includes: applying to a locus where plants are being grown or are expected to be grown either a recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention.

A sixth aspect of the invention relates to a method of imparting disease resistance to plants. This method includes: applying an effective amount of recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to impart disease resistance.

A seventh aspect of the invention relates to a method of enhancing plant growth. This method includes: applying an effective amount of recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to enhance plant growth.

An eighth aspect of the invention relates to a method of increasing a plant's tolerance and resistance to biotic stressors. This method includes: applying an effective amount of recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to increase the plant's tolerance and resistance to biotic stress factors selected from the group consisting of pests such as insects, arachnids, nematodes, weeds, and combinations thereof.

A ninth aspect of the invention relates to a method of increasing a plant's tolerance to abiotic stress. This method includes: applying an effective amount of recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to increase the plant's tolerance to abiotic stress factors selected from the group consisting of salt stress, water stress (including drought and flooding), ozone stress, heavy metal stress, cold stress, heat stress, nutritional stress (phosphate, potassium, nitrogen deficiency), bleaching and light-induced stress, and combinations thereof.

A tenth aspect of the invention relates to a method imparting desiccation resistance to cuttings removed from ornamental plants. This method includes: applying recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant or the locus where the plant is growing, wherein said applying is effective to impart desiccation resistance to cuttings removed from the ornamental plant.

An eleventh aspect of the invention relates to a method of imparting post-harvest disease or post-harvest desiccation resistance to a fruit or vegetable. This method includes: applying an effective amount of recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant containing a fruit or vegetable or the locus where the plant is growing; or applying an effective amount of the recombinant host cell or the composition to a harvested fruit or vegetable, wherein said applying is effective to impart post-harvest disease resistance or desiccation resistance to the fruit or vegetable.

A twelfth aspect of the invention relates to a method of enhancing the longevity of fruit or vegetable ripeness. This method includes: applying an effective amount of recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant containing a fruit or vegetable or the locus where the plant is growing; or applying an effective amount of the recombinant host cell or the composition to a harvested fruit or vegetable, wherein said applying is effective to enhance the longevity of fruit or vegetable ripeness.

A thirteenth aspect of the invention relates to a method of modulating one or more biological signaling processes of a plant. This method includes: applying an effective amount of recombinant host cell according to the first aspect of the invention, or a composition according to the second aspect of the invention to a plant or the locus where the plant is growing, wherein said applying is effective in modulating one or more biochemical signaling processes.

A growing aspect of the commercial crop protection market involves the use of living biological agents, including bacteria, fungi, and other beneficial microbes. These organisms may directly or indirectly antagonize plant pathogens through killing, competition for resources, and competition for space on plant surfaces. In addition, some beneficial microbes may set up a direct symbiotic relationship with the host plant. Since there are significant benefits to a grower in reducing the number of products applied to the field as well as reducing the total number of applications, the present invention affords many benefits to growers by using a long-lived, recombinant microorganism to produce a non-native harpin protein or effector peptide for inducing plant stimulation. Thus, in a single application a plant grower can obtain both the long-lasting benefits afforded by the microorganism and the harpin protein or effector peptide expressed by the microorganism.

DETAILED DESCRIPTION OF THE INVENTION

One aspect of the invention relates to a recombinant host cell comprising a transgene that comprises a promoter-effective nucleic acid molecule operably coupled to a nucleic acid molecule that encodes a plant effector protein or polypeptide, wherein the recombinant host cell is a microbe that imparts a first benefit to a plant grown in the presence of the recombinant microbe and the plant effector protein or polypeptide imparts a second benefit to the plant grown in the presence of the recombinant microbe.

The terms defined immediately below are more fully defined by reference to the specification as a whole.

The term “transgene” refers to a gene introduced into the beneficial microbe, making the beneficial microbe recombinant. The introduction of a transgene into the beneficial microbe has the potential to change the phenotype of that microbe, in the present case due to the expression of the plant effector protein or polypeptide by the recombinant beneficial microbe. The construction of a transgene involves the assembly of a few main parts, including a promoter sequence (defined below), a protein coding sequence (defined below), and a stop codon.

The term “promoter” is defined herein as a nucleic acid that directs transcription of a downstream polynucleotide in a cell. In certain cases, the polynucleotide may contain a coding sequence and the promoter may direct the transcription of the coding sequence into translatable RNA.

The term “coding sequence” is defined herein as a nucleic acid that, when placed under the control of appropriate control sequences including a promoter, is transcribed into mRNA which can be translated into a polypeptide. A coding sequence may contain a single open reading frame, or several open reading frames separated by introns, for example. A coding sequence may be cDNA, genomic DNA, synthetic DNA or recombinant DNA, for example. A coding sequence generally starts at a start codon (e.g., ATG) and ends at a stop codon (e.g., UAA, UAG and UGA).

The term “recombinant” refers to a polynucleotide or polypeptide that does not naturally occur in a host cell, as well as host cells that contain a non-naturally occurring polynucleotide or polypeptide. A recombinant molecule may contain two or more naturally occurring sequences that are linked together in a way that does not occur naturally. Thus, a “recombinant host cell” refers to a host cell that is non-naturally occurring, e.g., through the introduction of a recombinant polynucleotide (or transgene) into the host cell.

The term “operably coupled” refers to a juxtaposition, wherein elements are in an arrangement allowing them to be functionally related. For example, a promoter is operably linked to a coding sequence if it controls the transcription of the sequence, and a signal sequence is operably linked to a protein if the signal sequence directs the protein through the secretion system of a host cell. Generally, this operable linkage is reflected by the relative positioning of elements along a DNA strand.

The term “nucleic acid” encompasses DNA, RNA, single or doubled stranded and modification thereof. The terms “nucleic acid” and “polynucleotide” may be used interchangeability herein.

As used herein, the terms “polypeptide” and “protein” are used interchangeably and include reference to a polymer of any number of amino acid residues. The terms apply to amino acid polymers in which one or more amino acid residue is an artificial chemical analog of a corresponding naturally occurring amino acid, as well as to naturally occurring amino acid polymers. The terms also apply to polymers containing conservative amino acid substitutions such that the polypeptide remains functional. “Peptides” are polypeptides having less than 50 amino acid residues.

A “host cell” is a cell that contains a subject recombinant nucleic acid, either in the genome of the host cell or in an extrachromosomal vector that replicates autonomously from the genome of the host cell. A host cell may be any cell type.

In various embodiments, a host cell comprising a subject recombinant nucleic acid is provided. The host cell may be any cell type, but is preferably a microbe, e.g., a bacterial or fungal (such as a non-filamentous or filamentous fungal) host cell.

In certain embodiments, the microbe is a beneficial microbe that imparts a benefit to a plant grown in the presence of the microbe. A recombinant beneficial microbe also imparts a benefit to a plant grown in the presence of the microbe, but due to the presence of a recombinant polynucleotide the recombinant beneficial microbe also expresses a plant effector protein or polypeptide that imparts a second benefit to the plant grown in the presence of the recombinant microbe.

The term “filamentous fungi” refers to all filamentous forms of the subdivision Eumycotina (see Alexopoulos, C. J., INTRODUCTORY MYCOLOGY, Wiley, New York (1962), which is hereby incorporated by reference in its entirety). These fungi are characterized by a vegetative mycelium with a cell wall composed of chitin, glucans, and other complex polysaccharides. The filamentous fungi of the present invention are morphologically, physiologically, and genetically distinct from yeasts. Vegetative growth by filamentous fungi is by hyphal elongation and carbon catabolism is obligatory aerobic.

In certain embodiments, the beneficial microbe is a bacterium.

Suitable beneficial bacterium include, without limitation, Pseudomonas (e.g., P. fluorescens, P. aureofaciens, P. chlororaphis, P. solanacearum, and P. syringae), Sphingomonas (e.g., S. phyllosphaerae, S. roseiflava, S. melonis, S. azotifigens, and S. mali) (see also Innerebner et al., “Protection of Arabidopsis thaliana Against Leaf-Pathogenic Pseudomonas syringae by Sphingomonas Strains in a Controlled Model System,” Appl. Environ. Microbiol. 77:3202-3210 (2011), which is hereby incorporated by reference in its entirety), Bacillus (B. firmus, B. licheniformis, B. megaterium, B. mucilaginous, B. pumilus, B. subtilis, and B. subtilis var. amyloliquefaciens), Streptomyces (e.g., S. griseoviridis and S. lydicus), Rhizobium (e.g., R. meliloti, R. trifolii, R. leguminosarum, R. phaseolin, R. lupine, and R. japonicum), Frankia (e.g., F. alni), and Azospirillum (e.g., A. brasilense and A. lipoferum).

Additional beneficial bacterium, include, without limitation, Agrobacterium radiobacter, Azotobacter chroococcum, Burkholderia cepacia, Delfitia acidovorans, Paenobacillus macerans, Pantoea agglomerans, and Serratia entomophilia.

In certain embodiments, the host cell may be a filamentous fungal host cell. In some embodiments, the host cell may be a cell of a strain that has a history of use for production of proteins that has GRAS status, i.e., a Generally Recognized as Safe, by the FDA.

In some embodiments, subject fungal host cells may be of a strain of Aspergillus niger which include ATCC 22342, ATCC 44733, ATCC 14331, ATCC 11490, NRRL 3112, and strains derived therefrom. In some embodiments, subject fungal cells may be strains of Trichoderma (e.g. T. harzianum, T. viride, T. koningi, T. reesei and T. hamatum) which include functional equivalents of RL-P37 (Sheir-Neiss et al. Appl. Microbiol. Biotechnology 20:46-53 (1984), which is hereby incorporated by reference in its entirety). Other useful host strains include, without limitation, NRRL 15709, ATCC 13631, ATCC 26921 (QM 9414) ATCC 32098, ATCC 32086, and ATCC 56765 (RUT-30). In some embodiments, subject fungal cells may be strains of non-filamentous fungal yeasts, including, without limitation, strains of Rhodotorula (e.g., R. graminis WP1 and R. mucilaginosa) (see U.S. Pat. No. 8,728,781 and Xin et al., “Characterization of Three Endophytic, Indole-3-Acetic Acid-Producing Yeasts Occurring in Populus Trees,” Mycol. Res. 113:973-980 (2009), which are hereby incorporated by reference in their entirety).

In some embodiments, a host cell may be one wherein native genes have been deleted or inactivated. For example, genes corresponding to protease genes (e.g., aspartyl protease, (Berka et al. Gene 86:153-162 (1990) and U.S. Pat. No. 6,509,171, which are hereby incorporated by reference in their entirety)) or genes corresponding to cellulase genes (e.g., cbh1, cbh2 and egl1, and egl2) may be deleted or inactivated. One example of this is the quad deleted strain of T. reesei disclosed in PCT Application Publ. No. WO 05/001036, which is hereby incorporated by reference in its entirety.

In certain embodiments, the recombinant microbe is epiphytic. Such a microbe lives non-parasitically on the surface of the host plant tissues, including without limit, at the surface of leaves or near roots.

In other embodiments, the recombinant microbe is endophytic. Such a microbe lives at least part of its life-cycle non-parasitically within plant tissues, including without limit, within leaves, roots, and stems.

One aspect of the invention is a DNA molecule capable of directing production of the plant bioactive polypeptide or protein. This DNA molecule contains several component sequences. These include but are not limited to the sequence coding the open reading frame for the plant effector protein or polypeptide, a ribosome-binding sequence, and a promoter. Additional sequences may include a selectable marker and an origin of replication. Optional sequences include secretion signals and sequences for genomic integration.

The term “signal sequence” or “signal peptide” refers to a sequence of amino acids at the N-terminal portion of a protein, which facilitates the secretion of the mature form of the protein outside the host cell. The mature form of the extracellular protein lacks the signal sequence which is cleaved off during the secretion process.

A promoter sequence directs the recruitment of an RNA polymerase complex to the DNA template. The choice of promoter sequence determines the conditions under which the transgene will be transcribed to allow for protein expression. Promoter sequences differ between species as they must interact with host cell transcription factors. Although strong promoters are often preferred for protein expression during fermentation, the present invention is not limited to strong, exponential growth promoters. Weak promoters and promoters activated during stationary phase and slow-growth conditions are also appropriate.

A preferred constitutively active promoter sequence for B. subtilis is the aprE promoter sequence as described by Park et al., “Bacillus subtilis subtilisin gene (aprE) is expressed from a sigma A (sigma 43) promoter in vitro and in vivo,” J Bact. 171:2657-2665 (1989), which is hereby incorporated by reference in its entirety. Another preferred constitutively active weak promoter sequence is PliaG promoter as described by Jordan et al., “Regulation of LiaRS-dependent Gene Expression in Bacillus subtilis: Identification of Inhibitor Proteins, Regulator Binding Sites and Target Genes of a Conserved Cell Envelope Stress-sensing Two-component System,” J Bacteriol. 188: 5153-5166 (2006), which is hereby incorporated by reference in its entirety. Another preferred promoter sequence is the ctc promoter that is activated under nutrient and other stress conditions, as described by Igo and Losick, “Regulation of a Promoter That is Utilized by Minor Forms of RNA Polymerase Holoenzyme in Bacillus subtilis,” J Mol. Biol. 191: 615-624 (1986), which is hereby incorporated by reference in its entirety. More recently, additional tools have been developed for protein expression in B. subtilis, including a number of promoters, as summarized by Radeck et al., “The Bacillus BioBrick Box: Generation and Evaluation of Essential Genetic Building Blocks for Standardized Work with Bacillus subtilis,” J Biol. Eng. 7:29 (2013), which is hereby incorporated by reference in its entirety. Additional information is available online at the iGEM Registry of Standard Biological Parts (see http://parts.igem.org/Promoters/Catalog/B._subtilis/Constitutive and http://parts.igem.org/Bacillus_subtilis).

In certain embodiments, the polynucleotide may be codon optimized for expression of the protein in a particular host cell. Since codon usage tables listing the usage of each codon in many cells are known in the art (see, e.g., Nakamura et al, Nucl. Acids Res. 28: 292 (2000), which is hereby incorporated by reference in its entirety) or readily derivable, such nucleic acids can be readily designed giving the amino acid sequence of a protein to be expressed.

In addition to a coding sequence, the recombinant nucleic acid may in certain embodiments further contain other elements that are necessary for expression of the protein in the host cell. For example, the nucleic acid may contain a transcriptional terminator, and 5′ and 3′ UTR sequences. Suitable 5′ UTR sequences may be obtained from the T. reesei cbh1, cbh2, egl1, egl2, egl5, xln1 and xln2 genes, for example. Suitable terminators include the T. reesei cbh1, cbh2, egl1, egl2, egl5, xln1 and xln2 terminators, and many others, including, for example, the terminators from A. niger or A. awamori glucoamylase genes (Nunberg et al. Mol. Cell. Biol. 4: 2306-2353 (1984); Boel et al., EMBO J. 3:1097-1102 (1984), each of which is hereby incorporated by reference in its entirety), Aspergillus nidulans anthranilate synthase genes, Aspergillus oryzae TAKA amylase genes, or A. nidulans trpc (Punt et al., Gene 56:117-124 (1987), which is hereby incorporated by reference in its entirety). The promoter and/or terminator may be native or non-endogenous to the host cell. In certain cases, the promoter and protein coding sequence may be separated by a sequence encoding a 5′ untranslated region, for example.

As will be discussed in greater detail below, a subject recombinant nucleic acid may be present in a vector, or integrated into a genome (i.e., the nuclear genome) of a host cell.

The term “vector” is defined herein as a polynucleotide designed to carry nucleic acid sequences to be introduced into one or more cell types. Vectors include cloning vectors, expression vectors, shuttle vectors, plasmids, phage or virus particles, DNA constructs, cassettes and the like. Expression vectors may include regulatory sequences such as promoters, signal sequences, a coding sequences and transcription terminators.

An “expression vector” as used herein means a DNA construct comprising a coding sequence that is operably linked to suitable control sequences capable of effecting expression of a protein or polypeptide in a suitable host. Such control sequences may include a promoter to effect transcription, an optional operator sequence to control transcription, a sequence encoding suitable ribosome binding sites on the mRNA, enhancers and sequences which control termination of transcription and translation.

In certain embodiments, the expression vector comprises an origin of replication operable in the recombinant host cell.

The term “DNA construct” as used herein means a nucleic acid sequence that comprises at least two DNA polynucleotide fragments.

A subject recombinant nucleic acid may be present in a vector, e.g., a phage, plasmid, viral, or retroviral vector that autonomously replicates in a host cell. In certain embodiments, the vector may be an expression vector for expressing a protein or polypeptide in a host cell. In certain embodiments, the vector may be an expression vector for expressing a subject polypeptide in a filamentous fungal cell.

Vectors for expression of recombinant proteins are well known in the art (Ausubel, et al, Short Protocols in Molecular Biology, 3rd ed., Wiley & Sons (1995); Sambrook, et al., Molecular Cloning: A Laboratory Manual, Second Edition, (1989) Cold Spring Harbor, N.Y., each of which is hereby incorporated by reference in its entirety).

A subject vector may be constructed using well known techniques as is generally described for example in EP Application Publication 0215594, which is hereby incorporated by reference in its entirety. Once the fusion DNA construct is made it may be incorporated into any number of vectors as is known in the art. While the DNA construct will preferably include a promoter sequence, in some embodiments the vector will include regulatory sequences functional in the host to be transformed, such as promoters, ribosomal binding sites, transcription start and stop sequences, terminator sequences, polyadenylation signals, enhancers and/or activators.

Polypeptide expression systems can be created using existing plasmid systems by one skilled in the art. One notable guideline is that regulation of polypeptide expression should be well controlled. High polypeptide concentrations detected by the plant will likely trigger an intense immune response with widespread cell death characteristic of the hypersensitive response. In contrast, lower polypeptide expression levels should stimulate desired immunity while minimizing cell death. This effect may be further balanced by careful choice of secretion sequences. Expression of polypeptides in Pseudomonas fluorescens may be accomplished using the expression strains and tools described by Retallack et al., “Reliable protein production in a Pseudomonas fluorescens expression system,” Protein Expression and Purification 81:157-65 (2012), which is hereby incorporated by reference in its entirety. Expression of peptides in Bacillus subtilis can be accomplished through vectors utilizing a subtilisin (aprE) promoter system. This can optionally be augmented using signal peptides to direct secretion of the peptide outside of the microbe. These functions are implemented in the “Bacillus Subtilis Secretory Protein Expression System” manual available from Clontech, which is hereby incorporated by reference in its entirety. Expression of proteins in Streptomyces has been demonstrated using plasmids as described by Fernandez-Abalos et al., “Posttranslational Processing of the Xylanase Xys1L From Streptomyces halstedii JM8 is Carried Out by Secreted Serine Proteases,” Microbiology 149:1623-32 (2003), which is hereby incorporated by reference in its entirety. Additional peptide expression systems can be produced by one skilled in the art.

Depending on the species of microbe chosen, the inserted sequences may exist as a circular plasmid that is independently propagated within the cell. Briefly, a plasmid incorporates all of the necessary DNA sequences for protein expression along with the optional sequences described below. A plasmid also requires an origin of replication, which is necessary for replication and maintenance of the plasmid. Optionally, a plasmid can contain a second origin of replication specific for E. coli, including the well-known pMB1 origin of replication present in the pBR322 vector as described by Sutcliffe, “Complete Nucleotide Sequence of the Escherichia coli Plasmid pBR322,” Cold Spring Harb. Symp. Quant. Biol. 43: 77-90 (1979), which is hereby incorporated by reference. Other E. coli replication origins are known to one skilled in the art.

As an alternative to an independent plasmid, the expression sequences may be integrated into the genome of the host microbe. In certain organisms, notably fungi, this is accomplished by homologous recombination between sequences in a plasmid and the host genome. This requires that the heterologous plasmid contain host DNA sequences for mediation of the recombination event. Integration may also be accomplished using selection for a random non-homologous integration event or directed integration via genome editing techniques, including CRISPR-Cas9-directed integration as described by U.S. Pat. No. 8,871,445, which is hereby incorporated by reference in its entirety.

Although optional, inclusion of a selectable marker can speed development of transgenic organisms. One option for a selectable marker is the inclusion of an antibiotic resistance gene in bacteria, for instance: Ampicillin resistance by an expressed beta-lactamase enzyme or tetracycline resistance by an expressed drug efflux pump. Only cells containing the expression construct will survive challenge with the corresponding antibiotic. Examples of additional antibiotics include, but are not limited to, hygromycin, bleomycin, chloramphenicol and phleomycin). Additional antibiotics and corresponding resistance genes are known to one skilled in the art. Due to the ethical concerns of increased antibiotic use, alternative selection methods are preferred. These include the use of auxotrophic organisms. In this case, the microbe can be mutated by the removal of a biosynthetic gene for a required nutrient. Examples are genes associated with tryptophan, uracil, or adenine biosynthesis. The organism can grow on media supplemented with the nutrient, but cannot grow in conditions of a minimal medium that does not contain the nutrient. The expression construct is then modified with an intact copy of the missing biosynthetic gene (e.g. pyr4 complementation of a pyr4 deficient A. nidulans, A. awamori or Trichoderma reesei and argB complementation of an argB deficient strain). Reference is made to Kelley et al., EMBO J. 4: 475-479 (1985); Penttila et al., Gene 61:155-164 (1987) and Kinghom et al Applied Molecular Genetics of Filamentous Fungi, Blackie Academic and Professional, Chapman and Hall, London (1992), which are hereby incorporated by reference in their entirety. A final option is to include a toxin/anti-toxin system. Briefly, one gene encodes a long-lived toxin which will cause cell death. The toxin is bound and inactivated by an antitoxin protein. A cell containing a genomic copy of the toxin gene will die unless the cell also expresses the antitoxin protein. In general, the antitoxin protein is more highly-expressed as compared with the toxin protein, but it is also quickly degraded within the cell. The ratA/tpxA toxin system is endogenous to Bacillus subtilis as described by Silvaggi et al., “Small Untranslated RNA Antitoxin in Bacillus subtilis,” J Bacteriol. 187: 6641-6650 (2005), which is incorporated by reference in its entirety, and can control selection of a recombinant plasmid. Another bacterial toxin, GST-ParE, is disclosed in PCT Application Publ. No. WO/2002020750, which is hereby incorporated by reference in its entirety. Many other toxin/antitoxin systems are known in the art, as reviewed by Unterholzner et al., “Toxin-antitoxin systems: Biology, identification, and application,” Mobile Genetic Elements 3:5, e26219 (2013), which is hereby incorporated by reference in its entirety.

Another optional factor in the design of the expression construct is the choice of secretion signals for the peptide or protein. These signal sequences are added to the bioactive peptide or protein gene sequence and result in a fusion protein with a secretion tag sequence that directs localization of the active peptide through the host microbe's existing secretion machinery.

A library of secretion tags specific for Bacillus subtilis is available from Clontech as part of the Bacillus subtilis Secretory Protein Expression System; any one of these secretion tags can be used to direct secretion of a recombinant protein or polypeptide in B. subtilis.

One suitable secretion signal sequence for Trichoderma reesei is the CBH I secretion signal (MYRKLAVISAFLATARA, SEQ ID NO: 3) as described by Zhong et al., “Expression and Secretion of the Human Erythropoietin Using an Optimized cbh1 Promoter and the Native CBH I Signal Sequence in the Industrial Fungus Trichoderma reesei,” Appl. Biochem. Biotechnol. 165:1169-1177 (2011), which is hereby incorporated by reference in its entirety.

Terminator sequences which are recognized by the expression host to terminate transcription may be operably linked to the 3′ end of the fusion DNA construct encoding the fusion protein to be expressed. Those of general skill in the art are well aware of various terminator sequences that may be used with filamentous fungi. Non-limiting examples include the terminator from the Aspergillus nidulans trpC gene (Yelton M. et al., Proc. Natl. Acad. Sci. USA 81: 1470-1474 (1984), which is hereby incorporated by reference in its entirety) and the terminator from the Aspergillus niger glucoamylase genes (Nunberg et al., Mol. Cell. Biol. 4: 2306-2353 (1984), which is hereby incorporated by reference in its entirety). Likewise, transcriptional terminators for bacteria including E. coli, Bacillus subtilis, and others are known in the art. In particular, Bacillus terminators for the genes amyE, penP, and bglS have been characterized for efficacy by Hess and Graham, “Efficiency of transcriptional terminators in Bacillus subtilis,” Gene 95:137-41 (1990), which is hereby incorporated by reference in its entirety. Likewise, a bioinformatics approached revealed a large array of transcriptional terminators in B. subtilis and related species (de Hoon et al, “Prediction of transcriptional terminators in Bacillus subtilis and related species,” PLOS Comput. Biol. 1:e25 (2005), which is hereby incorporated by reference in its entirety. A similar study in E. coli showed the efficacy of the rrnB transcriptional terminator sequence (Lesnik et al., “Prediction of the rho-independent transcriptional terminators in Escherichia coli,” Nucleic Acids Research 29:3583-3594 (2001), which is hereby incorporated by reference in its entirety).

One exemplary DNA construct for expression in B. subtilis comprises the PliaG promoter fused with a B. subtilis codon-optimized synthetic gene containing the AmyE secretion signal fused N-terminal to the sequence of P15a (as described in U.S. patent application Ser. No. 14/872,298 to Wei et al. which is hereby incorporated by reference in its entirety) and the rho-independent transcriptional terminator from E. coli rrnB. Such a construct, further incorporating BamHI and XhoI sites for insertion into a DNA vector, is demonstrated by the DNA molecule of SEQ ID NO: 1 and the sequence annotation in FIG. 1. SEQ ID NO: 1 is reproduced below:

GGATCCCAAAAATCAGACCAGACAAAAGCGGCAAATGAATAAGCGGAACG GGGAAGGATTTGCGGTCAAGTCCTTCCCTTCCGCACGTATCAATTCGCAA GCTTTTCCTTTATAATAGAATGAATGAAAAGGAGGAAACAATCATGTTTG CAAAAAGATTTAAAACATGAGTGCTGCCGCTGTTTGCAGGCTTTCTGCTG CTGTTTCATCTGGTTCTGGCAGGCCCGGCAGCAGCATCAGCAGAAACAGC AAATAAATCAAATGAAAATTTTGGCACACCGGATTCAACAGTTCAAAATC CGCAAGATGCATCAAAACCGAATGATTCACAATCAAATATTGCAAAACTG ATTTCAGCACTGATTATGTCACTGCTGCAAATGTAACCAGGCATCAAATA AAACGAAAGGCTCAGTCGAAAGACTGGGCCTTTCGTTTTATCTGTTGTTT GTCGGTGAACGCTCTCGAG

One exemplary DNA construct for expression in Trichoderma reesei comprises a fusion of the cellobiosehydrolase I (CBH I) promoter with a secretion signal for cbhI, a synthetic codon-optimized P14 sequence (as described in U.S. patent application Ser. No. 14/872,347 to Wei et al., which is hereby incorporated by reference in its entirety) and the cbh1 terminator sequence from Trichoderma reesei. Such a construct, further incorporating XbaI and EcoRI sites for insertion into a DNA vector, is demonstrated by the DNA molecule of SEQ ID NO: 2 and the sequence annotation in FIG. 2. SEQ ID NO: 2 is reproduced below:

TCTAGAGTTGTGAAGTCGGTAATCCCGCTGTATAGTAATACGAGTCGCAT CTAAATACTCCGAAGCTGCTGCGAACCCGGAGAATCGAGATGTGCTGGAA AGCTTCTAGCGAGCGGCTAAATTAGCATGAAAGGCTATGAGAAATTCTGG AGACGGCTTGTTGAATCATGGCGTTCCATTCTTCGACAAGCAAAGCGTTC CGTCGCAGTAGCAGGCACTCATTCCCGAAAAAACTCGGAGATTCCTAAGT AGCGATGGAACCGGAATAATATAATAGGCAATACATTGAGTTGCCTCGAC GGTTGCAATGCAGGGGTACTGAGCTTGGACATAACTGTTCCGTACCCCAC CTCTTCTCAACCTTTGGCGTTTCCCTGATTCAGCGTACCCGTACAAGTCG TAATCACTATTAACCCAGACTGACCGGACGTGTTTTGCCCTTCATTTGGA GAAATAATGTCATTGCGATGTGTAATTTGCCTGCTTGACCGACTGGGGCT GTTCGAAGCCCGAATGTAGGATTGTTATCCGAACTCTGCTCGTAGAGGCA TGTTGTGAATCTGTGTCGGGCAGGACACGCCTCGAAGGTTCACGGCAAGG GAAACCACCGATAGCAGTGTCTAGTAGCAACCTGTAAAGCCGCAATGCAG CATCACTGGAAAATACAAACCAATGGCTAAAAGTACATAAGTTAATGCCT AAAGGAGTCATATACCAGCGGCTAATAATTGTACAATCAAGTGGCTAAAC GTACCGTAATTTGCCAACGGCTTGTGGGGTTGCAGAAGCAACGGCAAAGC CCCACTTCCCCACGTTTGTTTCTTCACTCAGTCCAATCTCAGCTGGTGAT CCCCCAATTGGGTCGCTTGTTTGTTCCGGTGAAGTGAAAGAAGACAGAGG TAAGAATGTCTGACTCGGAGCGTTTTGCATACAACCAAGGGCAGTGATGG AAGACAGTGAAATGTTGACATTCAAGGAGTATTTAGCCAGGGATGCTTGA GTGTATCGTGTAAGGAGGTTTGTCTGCCGATACGACGAATACTGTATAGT CACTTCTGATGAAGTGGTCCATATTGAAATGTAAGTCGGCACTGAACAGG CAAAAGATTGAGTTGAAACTGCCTAAGATCTCGGGCCCTCGGGCCTTCGG CCTTTGGGTGTACATGTTTGTGCTCCGGGCAAATGCAAAGTGTGGTAGGA TCGAACACACTGCTGCCTTTACCAAGCAGCTGAGGGTATGTGATAGGCAA ATGTTCAGGGGCCACTGCATGGTTTCGAATAGAAAGAGAAGCTTAGCCAA GAACAATAGCCGATAAAGATAGCCTCATTAAACGGAATGAGCTAGTAGGC AAAGTCAGCGAATGTGTATATATAAAGGTTCGAGGTCCGTGCCTCCCTCA TGCTCTCCCCATCTACTCATCAACTCAGATCCTCCAGGAGACTTGTAGAC CATCTTTTGAGGCACAGAAACCCAATAGTCAACCGCGGACTGGCATCATG TATCGGAAGTTGGCCGTCATCTCGGCCTTCTTGGCCACAGCTCAGGCCGG CCCCCAGAGCGCCAACAAGACCGGCAACGTCGACGACGCCAACAACCAGG ACCCCATGCAGGCCCTCATGCAGCTCCTCGAGGACCTCGTCTAAAGCTCC GTGCGAAAGCCTGACGCACCGGTAGATTCTTGGTGAGCCCGTATCATGAC GGCGGCGGGAGCTACATGGCCCCGGGTGATTTATTTTTTTTGTATCTACT TCTGACCCTTTTCAAATATACGGTCAACTCATCTTTCACTGGAGATGCGG CCTGCTTGGTATTGCGATGTTGTCAGCTTGGCAAATTGTGGCTTTCGAAA ACACAAAACGATTCCTTAGTAGCCATGCATTTTAAGATAACGGAATAGAA GAAAGAGGAAATTAAAAAAAAAAAAAAAACAAACATCCCGTTCATAACCC GTAGAATCGCCGCTCTTCGTGTATCCCAGTACCACGGCAAAGGTATTTCA TGATCGTTCAATGTTGATATTGTTCCCGCCAGTATGGCTCCACCCCCCAT CTCCGCGAATCTCCTCTTCTCGAACGCGGTGTGGCGCGCCAATTGGTAAT GACCCCATAGGGAGACAAACAGCATAATAGCAACAGTGGAAATTAGTGGC GAATTC

Introduction of a nucleic acid into a host cell includes techniques such as transformation; electroporation; nuclear microinjection; transduction; transfection, (e.g., lipofection mediated and DEAE-Dextrin mediated transfection); incubation with calcium phosphate DNA precipitate; high velocity bombardment with DNA-coated microprojectiles; and protoplast fusion. General transformation techniques are known in the art (see, e.g., Ausubel et al., (1987), supra, chapter 9; Sambrook (1989) supra; and Campbell et al., Curr. Genet. 16:53-56 (1989), which are hereby incorporated by reference in their entirety). Reference is also made to PCT Application Publ. No. WO 05/001036; U.S. Pat. Nos. 6,022,725; 6,103,490; 6,268,328; and published U.S. Application Publ. Nos. 20060041113, 20060040353, 20060040353 and 20050208623, which are incorporated herein by reference in their entirety.

“Transformation” means introducing DNA into a cell so that the DNA is maintained in the cell either as an extrachromosomal element or chromosomal integrant.

The expression of recombinantly introduced proteins in Trichoderma is described in U.S. Pat. Nos. 6,022,725; 6,268,328; Harkki et al. Enzyme Microb. Technol. 13:227-233 (1991); Harkki et al., Bio Technol. 7:596-603 (1989); EP Pat. No. 244,234; EP Pat. No. 215,594; and Nevalainen et al., “The Molecular Biology of Trichoderma and its Application to the Expression of Both Homologous and Heterologous Genes,” in MOLECULAR INDUSTRIAL MYCOLOGY, Eds. Leong and Berka, Marcel Dekker Inc., NY (1992), pp. 129-148), which are hereby incorporated by reference in their entirety. Reference is also made to Cao et al., Protein Sci. 9:991-1001 (2000); Yelton et al., Proc. Natl. Acad. Sci. 81:1470-1471 (1984); U.S. Pat. No. 6,590,078; and Berka, et al., in: APPLICATIONS OF ENZYME BIOTECHNOLOGY, Eds. Kelly and Baldwin, Plenum Press, NY (1991), which are hereby incorporated by reference in their entirety, for transformation of Aspergillus strains.

In one embodiment, the vector is a Trichoderma expression vector related to pTrex3g, which is described in detail in Example 6 of PCT Application Publ. No. WO 05/001036, which is hereby incorporated by reference in its entirety.

In one embodiment, the preparation of Trichoderma sp. for transformation involves the preparation of protoplasts from fungal mycelia. (See Campbell et al., Curr. Genet. 16:53-56 (1989), which is hereby incorporated by reference in its entirety). In some embodiments, the mycelia are obtained from germinated vegetative spores. Transformation and protein expression in Aspergillus and Trichoderma is further described in, for example U.S. Pat. Nos. 5,364,770; 6,022,725; and Nevalainen et al., The Molecular Biology of Trichoderma and its Application to the Expression of Both Homologous and Heterologous Genes, in MOLECULAR INDUSTRIAL MYCOLOGY, Eds. Leon and Berka, Marcel Dekker, Inc. (1992) pp. 129-148, which are hereby incorporated by reference in their entirety.

Production of bioactive peptides in Pseudomonas is derived from existing work aimed at heterologous protein production under fermentation conditions in Pseudomonas, as described by Retallack et al., “Reliable Protein Production in a Pseudomonas fluorescens Expression System,” Prot. Exp. Purif. 81: 157-165 (2012), which is hereby incorporated by reference in its entirety. Notably, many components of E. coli expression plasmids are also effective in Pseudomonas. Adaptation of such plasmids for use in beneficial microbes may require changing the promoter. In particular, Miksch and Dobrowolski, “Growth Phase-dependent Induction of Stationary-phase Promoters of Escherichia coli in Different Gram-negative Bacteria,” J Bacteriol. 177: 5374-5378 (1995), which is hereby incorporated by reference in its entirety, showed that the E. coli stationary phase promoters bolAp1 and fic are functional in Acetobacter methanolicus, Xanthomonas campestris, Pseudomonas putida, and Rhizobium meliloti.

An additional aspect of the invention is the production of bioactive proteins and peptides from fungal sources. For fungal gene expression, a plasmid DNA element can be introduced that integrates into the fungal genome by recombination. U.S. Pat. No. 8,044,192, which is hereby incorporated by reference in its entirety, discloses the Stp1 promoter that is active in Trichoderma reesei upon glucose exhaustion. The disclosed plasmid pPGamdS can be adapted for the production of bioactive protein or peptide expression in Trichoderma. More recently, the cbhII promoter was successfully developed for protein expression in Trichoderma by Meng et al., “Heterologous Protein Expression in Trichoderma reesei Using the cbhII Promoter,” Plasmid 70: 272-276 (2013), which is hereby incorporated by reference in its entirety.

A culture of cells is also provided. The culture of cells may contain a population of the above-described cells, and growth medium. The growth medium may contain glucose as a carbon source. In particular embodiments, glucose may be the sole carbon source of the growth medium. The growth medium may be free of a carbon source that is known to induce activity of cellulase gene expression (see, e.g., Ilmen et al, Applied and Environmental Microbiology 63: 1298-1306 (1997), which is hereby incorporated by reference in its entirety). For example, the growth medium may be free of cellulose, lactose, sophorose, cellobiose, and/or other sugar or cellulose-related material that induces cellulase expression. The culture of cells may be at a temperature of about 30° C. (e.g., 27-33° C.), or at a temperature of about 37° C. (e.g., 34-39° C.), for example. In a particular embodiment, the growth medium may contain glucose, glucose and sopohorose, or lactose as a carbon source, and the culture may be grown at 30° C. or 37° C.

As noted above, the transgene expressed by the recombinant beneficial microbe is one that encodes a plant effector protein or polypeptide, which imparts a benefit to a plant grown in the presence of the recombinant beneficial microbe. The benefit imparted by the plant effector protein or polypeptide is distinct of the benefit imparted by recombinant beneficial microbe (i.e., in its naturally occurring, non-recombinant form).

In certain embodiments, the plant effector protein or polypeptide is selected from the group consisting of a hypersensitive response elicitor protein or polypeptide fragment thereof, modified peptides derived from these hypersensitive response elicitor protein or polypeptide fragments, a bacterial flagellin protein or polypeptide, an elongation factor Tu protein or polypeptide, a transglutaminase protein or polypeptide, a fungal elicitor protein or polypeptide, a plant pathogenesis-related (or PR) protein or polypeptide fragment thereof, a plant elicitor protein or polypeptide.

A protein is considered plant bioactive if treatment of any plant tissue with the peptide causes a biochemical signaling cascade within the plant. This can result from, without limit, the specific recognition of a peptide by a receptor embedded in the plant cell membrane, import or translocation of the protein into the plant cell and recognition by a cytoplasmic receptor, or recognition of other physical interactions such as the formation of pore in the plant cell membrane. This signaling cascade may either cause a change in gene expression or the release of signaling molecules from the cell. Changes in gene expression manifest as altered RNA concentrations, detectable by qRT-PCR or microarray experiments. The released signaling molecules can be, without limit, ethylene, jasmonic acid and related metabolites, salicylic acid, gibberellins, auxin, abscisic acid, reactive oxygen species, or potassium and hydronium ions (indicated by a pH change). In some cases, the chemical signaling and gene expression changes may cause an observable change in the appearance of a plant tissue. For example, the hypersensitive response as described by Wei et al., Science 257:85-88 (1992), which is hereby incorporated by reference in its entirety, is characterized by coordinated cell death that causes a browning and wilting of the affected tissues.

In certain embodiments, the plant effector protein or polypeptide is a hypersensitive response elicitor polypeptide fragment that induces a hypersensitive response in a plant to which the hypersensitive response elicitor polypeptide fragment is applied.

One representative class of peptides and proteins are the harpins and HR-box family of peptides, as described in U.S. patent application Ser. No. 14/872,298 to Wei et al. (specifically, Tables 1-10 therein), which is hereby incorporated by reference in its entirety. Another exemplary class of peptides is the family of peptides described in the U.S. Provisional Patent Application Ser. No. 62/319,138, filed Apr. 6, 2016, entitled “Hypersensitive Response Elicitor-Derived Peptides and Use Thereof (specifically, HR-eliciting peptides shown in Tables 1, 2, and 4, including without limitation SEQ ID NOS: 8-12, 20, 29, 30, 33, 34, 42-44, 50, 55-57, 71, 72, and 139 as identified therein), which is hereby incorporated by reference in its entirety. These cause a hypersensitive response when infiltrated into tobacco leaves.

Specific families of peptides disclosed in U.S. patent application Ser. No. 14/872,298 to Wei et al., incorporated by reference in the preceding paragraph, include:

-   (i) SXGISEKXXDXXXXXXXXAXXXP (identified therein as SEQ ID NO: 2 or     P4 consensus; SEQ ID NO: 19 herein), wherein     -   X at position 2 is Q, E, gamma-glutamate (“γ-glutamate”), G, A,         or S;     -   X at position 8 is Q, E, γ-glutamate, G, A, or S;     -   X at position 9 is L, A, D, isoaspartic acid (“isoD”), I, V, or         F;     -   X at position 11 is Q, E, γ-glutamate, G, A, or S;     -   X at position 12 is L, D, isoD, I, or F;     -   X at position 13 is L, I, V, or F;     -   X at position 14 is any hydrophilic amino acid, preferably C, S,         or T, S or T, or only S;     -   X at position 15 is Q, E, γ-glutamate, G, A, S, K, or I;     -   X at position 16 is L, A, I, V, M, or F;     -   X at position 17 is I, S, or F;     -   X at position 18 is Q, E, γ-glutamate, G, A, or S;     -   X at position 20 is L, I, V, or F;     -   X at position 21 is L or F; and     -   X at position 22 is Q, E, γ-glutamate, G, A, or S; -   (ii) XXGISEKXLDXLLTXLIXALLXX (identified therein as SEQ ID NO: 3 or     P1 consensus; SEQ ID NO: 20 herein), wherein     -   X at position 1 is N, D, isoD, G, A, or S;     -   X at position 2 is Q, E, γ-glutamate, G, A, or S;     -   X at position 8 is Q, E, γ-glutamate, G, A, or S;     -   X at position 11 is Q, E, γ-glutamate, G, A, or S;     -   X at position 15 is Q, E, γ-glutamate, G, A, or S;     -   X at position 18 is M, T, K, E, γ-glutamate, G, A, or S;     -   X at position 22 is Q, E, γ-glutamate, G, A, or S; and     -   X at position 23 is Q, E, γ-glutamate, G, A, or S; -   (iii) (L/M)XXLLXXLLXXLL (identified therein as SEQ ID NO: 25 or     P17/18 min consensus; SEQ ID NO: 21 herein), wherein     -   X at position 2 is A, S, T, G, D, isoD, E, γ-glutamate, Q, N, K,         or R;     -   X at position 3 is Q, A, S, T, G, D, isoD, E, γ-glutamate, N, K,         or R;     -   X at position 6 is A, S, T, G, D, isoD, E, γ-glutamate, Q, N, K,         or R;     -   X at position 7 is Q, A, S, T, G, D, isoD, E, γ-glutamate, N, K,         or R;     -   X at position 10 is K, A, S, T, G, D, isoD, E, γ-glutamate, Q,         N, or R; and     -   X at position 11 is S, A, T, G, D, isoD, E, γ-glutamate, Q, N,         K, or R; -   (iv) XXXXXXXXXXX(L/M)XXLLXXLLXXLLXXX (SEQ ID NO: 49, P17/18     consensus), wherein     -   X at position 1 is Q, S, E, γ-glutamate, A, T, G, D, isoD, N, K,         or R;     -   X at position 2 is Q, S, E, γ-glutamate, A, T, G, D, isoD, N, K,         or R;     -   X at position 3 is P, Q, S, E, γ-glutamate, A, T, G, D, isoD, N,         K, or R;     -   X at position 4 is I, Q, S, E, γ-glutamate, A, T, G, D, N, isoD,         K, or R;     -   X at position 5 is D, isoD, S, E, γ-glutamate, A, T, G, N, Q, K,         or R;     -   X at position 6 is R, Q, S, E, γ-glutamate, A, T, G, D, isoD, N,         or K;     -   X of position 7 is Q, S, E, γ-glutamate, A, T, G, D, isoD, N, K,         or R;     -   X at position 8 is T, Q, S, E, γ-glutamate, A, G, D, isoD, N, K,         or R;     -   X at position 9 is I, Q, S, E, γ-glutamate, A, T, G, D, isoD, N,         K, or R;     -   X at position 10 is E, γ-glutamate, Q, S, A, T, G, D, isoD, N,         K, or R;     -   X at position 11 is Q, S, E, γ-glutamate, A, T, G, D, isoD, N,         K, or R;     -   X at position 13 is A, S, T, G, D, isoD, E, γ-glutamate, Q, N,         K, or R;     -   X at position 14 is Q, A, S, T, G, D, isoD, E, γ-glutamate, N,         K, or R;     -   X at position 17 is A, S, T, G, D, isoD, E, γ-glutamate, Q, N,         K, or R;     -   X at position 18 is Q, A, S, T, G, D, isoD, E, γ-glutamate, N,         K, or R;     -   X at position 21 is K, A, S, T, G, D, isoD, E, γ-glutamate, Q,         N, or R;     -   X at position 22 is S, A, T, G, D, isoD, E, γ-glutamate, Q, N,         K, or R;     -   X at position 25 is S, A, T, G, D, isoD, E, γ-glutamate, Q, N,         K, or R;     -   X at position 26 is P, S, A, T, G, D, isoD, E, γ-glutamate, Q,         N, K, or R;     -   X at position 27 is Q, S, A, T, G, D, isoD, E, γ-glutamate, N,         K, or R; and     -   wherein one or more of amino acids 1 to 11 and/or 25 to 27 is         optionally not present; -   (v) XLXX(L/M)LXLIXX(L/I/V/F/M)(L/I/V/F/M) (identified therein as SEQ     ID NO: 26 or P19 consensus; SEQ ID NO: 22 herein), wherein     -   X at position 1 is optional and can be L, I, V, F, or M;     -   X at position 3 is K, A, S, T, G, D, isoD, E, γ-glutamate, Q, N,         or R;     -   X at position 4 is A, S, T, G, D, isoD, E, γ-glutamate, Q, N, K,         or R;     -   X at position 7 is K, A, S, T, G, D, isoD, E, γ-glutamate, Q, N,         or R;     -   X at position 10 is A, S, T, G, D, isoD, E, γ-glutamate, Q, N,         K, or R; and     -   X at position 11 is R, A, S, T, G, D, isoD, E, γ-glutamate, Q,         N, or K.         Specific peptides in Tables 1-10 of U.S. patent application Ser.         No. 14/872,298 to Wei et al. include the following peptides:

P1-18t (identified NQGISEKQLDQLLT (SEQ ID NO: 23) as SEQ ID NO: 42) QLITALLQQ P4-14s (identified SQGISEKQLDQLLS (SEQ ID NO: 24) as SEQ ID NO: 6) QLIQALLQP P18 (identified as QQPIDRQTIEQMAQ (SEQ ID NO: 25) SEQ ID NO: 83 LLAQLLKSLLSPQ P19 (identified as ITPDGQGGGQIGDN (SEQ ID NO: 26) SEQ ID NO: 89) PLLKAMLKLIA P30-3 (identified as LEELLEELIEELLE (SEQ ID NO: 27) SEQ ID NO: 190) E P30-4 (identified as LEELLEELIEELL (SEQ ID NO: 28). SEQ ID NO: 210)

In other embodiments, the plant effector protein or polypeptide is a hypersensitive response elicitor polypeptide fragment that induces an active plant response other than a hypersensitive response when the polypeptide fragment is applied. An exemplary class of peptides is the family of peptides described in patent application Ser. No. 14/872,347 to Wei et al. (specifically, Tables 1-16 therein), which is hereby incorporated by reference in its entirety. Another exemplary class of peptides is the family of peptides described in the U.S. Provisional Patent Application Ser. No. 62/319,138, filed Apr. 6, 2016, entitled “Hypersensitive Response Elicitor-Derived Peptides and Use Thereof (specifically, HR-negative peptides shown in Tables 1, 2, and 4, including without limitation SEQ ID NOS: 13, 15-19, 25-28, 51-53, and 140 as identified therein), which is hereby incorporated by reference in its entirety. Although these do not cause a hypersensitive response, they stimulate the production of hydrogen peroxide and other reactive oxygen species within tobacco or soy leaves.

Specific families of peptides disclosed in U.S. patent application Ser. No. 14/872,347 to Wei et al., incorporated by reference in the preceding paragraph, include those having a truncated HR Box sequence according to:

L-X-X-(L/I)-(L/I)-X-X-(L/I/V)-(L/I/V) (identified therein as SEQ ID NO: 116; SEQ ID NO: 29 herein), wherein

-   -   the peptide is less than 50 amino acids in length, and is free         of cysteine and methionine; each X at positions 2, 3, 6, 7 is         independently selected from the group consisting of G, A, S, T,         D, isoD, E, γ-glutamate, Q, N, K, and R; and     -   the peptide induces an active plant response, but does not         induce a hypersensitive response, when applied to mechanically         disrupted plant tissue.         Specific peptides in Tables 1-16 of U.S. patent application Ser.         No. 14/872,347 to Wei et al. include the following peptides:

P1-29 (identified NQGISEKQLDQLL (SEQ ID NO: 30) as SEQ ID NO: 130) TQLI P4-111 (identified SQGISEKQLDQLL (SEQ ID NO: 31) as SEQ ID NO: 132) SQLI P14 (identified as QAGPQSANKTGNV (SEQ ID NO: 32) SEQ ID NO: 113) DDANNQDPMQALM QLLEDLV P14a (identified as ANNQDPMQALMQL (SEQ ID NO: 33). SEQ ID NO: 114) LEDLV

Specific families of peptides disclosed in U.S. Provisional Patent Application Ser. No. 62/319,138, incorporated by reference in several paragraphs above, include:

-   (i) L-X-X-L-L-L-X-(F/L)-(I/L)-X-X-X-L (identified therein as SEQ ID     NO: 2; SEQ ID NO:

34 herein) wherein

-   -   X at position 3 is optional and, when present, is selected from         D, isoD, E, γ-glutamate, Q, N, S, and G, and     -   each X at positions 2, 7, 10, 11, and 12 is independently         selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G; or

-   (ii)     (Q/E)-(Q/E)-(L/I/V/F)-X-X-(L/I/V/F)-(L/I/V/F)-(L/I/V/F)-X-(L/I/V/F)-(L/I/V/F)-X-X-X-(L/I/V/F)-(D/G/Q/E)-(D/G/Q/E)     (identified therein as SEQ ID NO: 3; SEQ ID NO: 35 herein) wherein     -   X at position 5 is optional and, when present, is selected from         D, isoD, E, γ-glutamate, Q, N, S, and G, and     -   each X at positions 4, 9, 12, 13, and 14 is independently         selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G; or

-   (iii)     (L/I/V/F)-X-X-(L/I/V/F)-(L/I/V/F)-(L/I/V/F)-X-(L/I/V/F)-(L/I/V/F)-X-X-X-(L/I/V/F)-(D/G/Q/E)-(D/G/Q/E)     (identified therein as SEQ ID NO: 4; SEQ ID NO: 36 herein) wherein     -   X at position 3 is optional and, when present, is selected from         D, isoD, E, γ-glutamate, Q, N, S, and G, and     -   each X at positions 2, 7, 10, 11, and 12 is independently         selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G; or

-   (iv)     (Q/E)-(Q/E)-(L/I/V/F)-X-X-(L/I/V/F)-(L/I/V/F)-(L/I/V/F)-X-(L/I/V/F)-(L/I/V/F)-X-X-X-(L/I/V/F),     (identified therein as SEQ ID NO: 5; SEQ ID NO: 37 herein) wherein     -   X at position 5 is optional and, when present, is selected from         D, isoD, E, γ-glutamate, Q, N, S, and G, and     -   each X at positions 4, 9, 12, 13, and 14 is independently         selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G.         Specific peptides in Tables 1, 2, and 4 of U.S. Provisional         Patent Application Ser. No. 62/319,138 include the following         peptides:

P5 (identified as SAGSEQQLDLLLM (SEQ ID NO: 38) SEQ ID NO: 8) FIMMMLQQ P5a (identified as SAGSEQQLDQLLL (SEQ ID NO: 39) SEQ ID NO: 9) MFIMMMLQQ P5-21 (identified as SEEQLELLLAFIA (SEQ ID NO: 40) SEQ ID NO: 33) AALQQEE P5-25 (identified as SEEEEQLDQLLLA (SEQ ID NO: 41). SEQ ID NO: 52) FIAAALQQ Of these peptides, P5, P5a, and P5-21 are capable of inducing a hypersensitive response, whereas P5-25 does not.

Each of U.S. patent application Ser. No. 14/872,298 to Wei et al., U.S. patent application Ser. No. 14/872,347 to Wei et al., and U.S. Provisional Patent Application Ser. No. 62/319,138 also describes the expression of variants of the disclosed peptides, which can be recombinantly produced and then purified. The resulting variants differ from the disclosed peptides by the substitution of individual amino acids at enzymatic cleavage sites, which avoids the possibility of internal peptide cleavage upon exposure to a particular enzyme. One enzymatic cleavage site identified in all three of these applications is a trypsin specific cleavage site, which cleaves after Lys and Arg residues. U.S. patent application Ser. No. 14/872,298 to Wei et al. and U.S. patent application Ser. No. 14/872,347 to Wei et al. both provide an exemplary description of such variants, which involves mutating lysine and arginine residues to glutamate and introducing an arginine residue at the C-terminal end of the peptide. So mutated variants of SEQ ID NOS: 23-26 and 30-32 are shown below as SEQ ID NOS: 42-48

K→E P1-18t variant NQGISEEQLDQLLT (SEQ ID NO: 42) QLITALLQQR K→E P4-14s variant SQGISEEQLDQLLS (SEQ ID NO: 43) QLIQALLQPR K/R→E P18 variant QQPIDEQTIEQMAQ (SEQ ID NO: 44) LLAQLLESLLSPQR K→E P19 variant ITPDGQGGGQIGDN (SEQ ID NO: 45) PLLEAMLELIAR K→E P1-29 variant NQGISEEQLDQLLT (SEQ ID NO: 46) QLIR K→E P4-111 variant SQGISEEQLDQLLS (SEQ ID NO: 47) QLIR K→E P14 variant QAGPQSANETGNVD (SEQ ID NO: 48). DANNQDPMQALMQL LEDLVR

Peptides that are identified to “consist essentially of” a recited sequence include the recited amino acid sequence(s) optionally with one or more extraneous amino acids at the N- and/or C-terminal ends thereof, which extraneous amino acids do not materially alter one or more of the following properties: (i) the ability of the peptide to induce a hypersensitive response in plants, (ii) solubility of the peptide in water or aqueous solutions, (iii) stability of the peptide dissolved in water or aqueous solution at 50° C. over a period of time (e.g., 3 weeks), and (iv) resistance of the peptide to chemical degradation in the presence of an aqueous buffered solution that includes a biocidal agent (e.g., Proxel®GXL) at 50° C. over a period of time (e.g., 3 weeks). In certain embodiments, material alteration of the one or more properties is intended to mean that there is less than 20% variation, less than 15% variation, less than 10% variation, or less than 5% variation in a recited property when comparing a peptide possessing the one or more extraneous amino acids to an otherwise identical peptide lacking the one or more extraneous amino acids. In certain embodiments, the number of extraneous amino acids at the N- or C-terminal ends is up to 20 amino acids at one or both ends, up to 15 amino acids at one or both ends, up to 10 amino acids at one or both ends, up to 7 amino acids at one or both ends, up to 5 amino acids at one or both ends, or up to 3 amino acids at one or both ends. Further, to the extent that a recited sequence is in the form of a consensus sequence where one or more of the denoted X or Xaa residues can be any of one or more amino acids, then multiple peptide sequences are embraced by the peptide consisting essentially of such a recited sequence, without regard to additional variations of such sequences that are afforded by the presence of extraneous amino acids at the N- and/or C-terminal ends thereof.

A number of peptides are described in the art as inducing a response in plant cells. Flg22 is a 22-amino acid peptide sequence from the bacterial flagellin protein that causes a response in tomato cells as shown by Felix et al., “Plants Have a Sensitive Perception System For the Most Conserved Domain of Bacterial Flagellin,” Plant j. 18: 265-76 (1999), which is hereby incorporated by reference in its entirety. Elf18 is a peptide derived from elongation factor Tu that likewise causes an immune response in the cells of Arabidopsis thaliana, as shown by Kunze et al., “The N Terminus of Bacterial Elongation Factor Tu Elicits Innate Immunity in Arabidopsis Plants,” Plant Cell 16: 3496-3507 (2004) which is hereby incorporated by reference in its entirety. There are also proteins of fungal origin known to induce a response in plant cells. Pep-13 is a peptide sequence from a transglutaminase protein of the pathogenic Phytophthora sojae that causes a response in parsley and potato cells as shown by Brunner et al., “Pep-13, a Plant Defense-inducing Pathogen-associated Pattern From Phytophthora Transglutaminases,” EMBO J 21:6681-6688 (2002), which is hereby incorporated by reference in its entirety. Further, proteins PevD1 from Verticillium dahliae and PebC1 from Botrytis cinerea induce responses in cotton and Arabidopsis, respectively (Bu et al. “A Fungal Protein Elicitor PevD1 Induces Verticillium Wilt Resistance in Cotton,” Plant Cell Rep. 33: 461-470 (2014) and Zhang et al. “Fungal Elicitor Protein PebC1 From Botrytis cinerea Improves Disease Resistance in Arabidopsis thaliana,” Biotechnolo. Lett. 36:1069-1078 (2014), which are hereby incorporated by reference in their entirety). A 28-amino acid peptide derived from the Avr9 gene of Cladosporum fulvum that causes a response in certain cultivars of tomato, as shown by Van den Ackerveken et al. “The AVR9 Race-specific Elicitor of Cladosporium fulvum is Processed by Endogenous and Plant Proteases,” Plant Physiol. 103: 91-96 (1993), which is hereby incorporated by reference in its entirety. Additional pathogen proteins and peptides can also mediate plant defenses that are known to one skilled in the art.

Some plant-derived peptides are capable of inducing plant immune responses. The first of these to be described was Systemin, a small peptide from tomato leaves, described in U.S. Pat. No. 5,378,819, which is hereby incorporated by reference in its entirety. More recently, peptide sequences initially derived from Arabidopsis were found to exist in a variety of crop species, as described in U.S. Pat. Nos. 8,686,224 and 9,109,039, which are hereby incorporated by reference in their entirety. Additional members of this family are described by Lori et al. “Evolutionary Divergence of the Plant Elicitor Peptides (Peps) and Their Receptors: Interfamily Incompatibility of Perception but Compatibility of Downstream Signaling” J Exp. Bot. 66: 5315-5325 (2015), which is hereby incorporated by reference in its entirety. Additional peptides have also been discovered in soy plants, including GmSubPep, Gmpep914, Gmpep890, as described by Pearce et al., “A Subtilisin-like Protein From Soybean Contains an Embedded, Cryptic Signal That Activates Defense-related Genes,” PNAS 107:14921-14925 (2010) and Yamaguchi et al., “GmPep914, an Eight-Amino Acid Peptide Isolated From Soybean Leaves, Activates Defense-related Genes,” Plant Physiol. 156: 932-942 (2011), which are hereby incorporated by reference in their entirety.

The benefits attributable to the use of the recombinant beneficial microbe depend on the type of microbe and the plant effector protein expressed thereby. In certain embodiments, the benefit attributable to the recombinant beneficial microbe is providing nutrients to a plant, producing plant hormone analogs that stimulate growth or reduce stress signaling, or competing with pathogenic organisms. In certain embodiments, the benefit attributable to the plant effector protein or polypeptide is improved disease resistance, growth enhancement, tolerance and resistance to biotic stressors, tolerance to abiotic stress, desiccation resistance for cuttings removed from ornamental plants, post-harvest disease resistance or desiccation resistance to fruit or vegetables harvested from plants, and/or improved longevity of fruit or vegetable ripeness for fruit or vegetables harvested from plants. Multiple different recombinant host cells can be used in combination.

Once engineered microbes are raised, e.g., in a fermentation apparatus, the engineered microbes can be recovered and then provided in either a dry composition or a liquid composition or suspension. Thus, a further aspect of the invention relates to a composition that includes a plurality of recombinant host cells as described above and one or more carriers. The plurality of recombinant host cells can be the same type, e.g., conferring the same benefits to plants grown in their presence, or the plurality of recombinant host cells can include a plurality of distinct recombinant host cells that each confer distinct combinations of benefits to plants grown in their presence.

Colony forming units (c.f.u.) are used to quantify microbes. 1 c.f.u. of a microbe generates a single colony when spread onto a solid nutrient agar compatible with the organism and corresponds to one healthy, replication competent cell. In a dry powder formulation, the concentration of microbes can exceed 5×10¹⁰ cfu/gram of material. Suitable concentrations for a dry formulation include >10¹¹, >5×10¹⁰, >10¹⁰, >10⁹, >10⁸, 10⁷, or 10⁶ cfu/gram. Likewise, microbes can be provided as a liquid suspension. Suitable concentrations for a liquid formulation include >10¹⁰, >10⁹, >10⁸, >10⁷, >10⁶, >10⁵ cfu/ml.

Suitable carriers include water, aqueous solutions optionally containing one or more co-solvents, slurries, and solid carrier particles. Exemplary solid carriers include mineral earths such as silicates, silica gels, talc, kaolins, limestone, lime, chalk, bole, loess, clays, dolomite, diatomaceous earth, calcium sulfate, magnesium sulfate, magnesium oxide, ground synthetic materials, and products of vegetable origin, such as cereal meal, tree bark meal, wood meal and nutshell meal, cellulose powders, starches and starch derivatives, as well as other mono-, di-, and poly-saccharides. Exemplary aqueous solutions include those having pH 6-8, more preferably 6.5 to 7.5, containing a buffer matched to this range. Suitable buffers include, without limitation citrate, phosphate, carbonate, and HEPES. However, some microbes can persist in a spore form that is more resilient extremes of heat and pH as well as extended storage. Exemplary aqueous solutions compatible with this spore state include those having pH 3-8, more preferably 4.0-7.5, containing a buffer matched to this range. In addition to buffers described supra, suitable buffers include, without limitation, acetate, glutamate, and aspartate. The solution may optionally be supplemented with an enzymatic digest of proteins, yeast extract, and mineral nutrients, including but not limited to magnesium and iron.

Other suitable additives include buffering agents, wetting agents, coating agents, and abrading agents. These materials can be used to facilitate application of the compositions in accordance with the present invention.

For liquid compositions or suspensions, the microbes can be mixed in water, or a buffer solution, and applied as a spray or soaking treatment to the plant seeds, the plants or the locus where plants are grown. Alternatively, the solution can be applied prior to planting seeds at the locus, after planting seeds at the locus, prior to planting one or more seedlings at the locus, after planting one or more seedlings at the locus, or to the locus while plants are being grown at the locus.

For dry compositions, the microbes can be dried with or without inert carrier particles, and the dry composition can be applied to seeds, the locus where seeds will be planted or plants are being grown, or directly to plants.

As discussed hereinafter, the recombinant beneficial microbes can be used to impart multiple benefits to plants grown in the presence of the recombinant beneficial microbes. These uses involve application of the recombinant beneficial microbes directly to plant seeds, directly onto plants, or indirectly onto plants via application to the locus where seeds will be plants or plants are being grown. In these embodiments, the locus may include artificial or natural soil, a polymer growth medium, or a hydroponic growth medium. The soil can be present in any of a variety of environments including an open field, a partially covered field, a greenhouse, etc.

The present invention further relates to methods of imparting disease resistance to plants, enhancing plant growth, effecting pest control, imparting biotic or abiotic stress tolerance to plants, and/or modulating plant biochemical signaling. According to one embodiment, these methods involve applying an effective amount of recombinant host cell of the invention, or a composition of the invention to a plant or plant seed or the locus where the plant is growing or is expected to grow. As a consequence of such application, the recombinant host cell contacts cells of the plant or plant seed, and induces in the plant or a plant grown from the plant seed disease resistance, growth enhancement, tolerance to biotic stress, tolerance to abiotic stress, or altered biochemical signaling. According to an alternative embodiment, the recombinant host cell or composition of the invention can be applied to plants such that seeds recovered from such plants themselves are able to impart disease resistance in plants, to enhance plant growth, to affect insect control, to impart tolerance to biotic or abiotic stress, and/or to modulate biochemical signaling, to modulate maturation.

In these embodiments, it is also possible to select plants or plant seeds or the locus to which the recombinant host cell or composition of the invention is applied. For example, for fields known to contain a high nematode content, the plants or plant seeds to be grown in such fields, or the fields (locus), can be selectively treated by applying the recombinant host cell or composition of the invention as described herein; whereas no such treatment may be necessary for plants or plant seeds grown in fields containing low nematode content. Similarly, for fields having reduced irrigation, the plants or plant seeds to be grown in such fields, or the fields (locus), can be selectively treated by applying the recombinant host cell or composition of the invention as described herein; whereas no such treatment may be necessary for plants or plant seeds grown in fields having adequate irrigation. Likewise, for fields prone to flooding, the plants or plant seeds to be grown in such fields, or the fields (locus), can be selectively treated by applying the recombinant host cell or composition of the invention as described herein; whereas no such treatment may be necessary for plants or plant seeds grown in fields that are not prone to flooding. As yet another example of such selection, for fields prone to insect attack at certain times of the growing season, the plants or plant seeds to be grown in such fields, or the fields (locus), can be selectively treated by applying the recombinant host cell or composition of the invention as described herein; whereas the same field may not be treated at ineffective times of the growing season or other fields that are not prone to such attack may go untreated. Such selection steps can be carried out when practicing each of the methods of use described herein, i.e., imparting disease resistance to plants, enhancing plant growth, effecting pest control (including insects and nematodes), imparting biotic or abiotic stress tolerance to plants, and/or modulating plant biochemical signaling.

The present invention further relates to methods of improving desiccation resistance for cuttings removed from ornamental plants, post-harvest disease resistance or desiccation resistance to fruit or vegetables harvested from plants, and/or improved longevity of fruit or vegetable ripeness for fruit or vegetables harvested from plants. These methods involve applying an effective amount of recombinant host cell of the present invention or a composition according to the present invention to a plant or the locus where the plant is growing. As a consequence of such application, the recombinant host cell contacts cells of the plant or plant seed, and induces desiccation resistance for cuttings removed from ornamental plants, post-harvest disease resistance or desiccation resistance to fruit or vegetables harvested from plants, and/or improved longevity of fruit or vegetable ripeness for fruit or vegetables harvested from plants. Alternatively, an effective amount of recombinant host cell of the present invention or a composition according to the present invention can be applied to a harvested fruit or vegetable. As a consequence of such application, the recombinant host cell contacts cells of the harvested fruit or vegetable, and induces post-harvest disease resistance or desiccation resistance to the treated fruit or vegetables, and/or improved longevity of fruit or vegetable ripeness for the treated fruit or vegetables.

In these embodiments, it is also possible to select plants, cuttings, fruits, vegetables, or the locus to which the recombinant host cell or composition of the invention is applied. For example, for harvested cuttings or fruit or vegetables that are being shipped great distances or stored for long periods of time, then these can be selectively treated by applying the recombinant host cell or composition of the invention as described herein; whereas harvested cuttings or fruit or vegetables that are being shipped locally and intended to be consumed without substantially periods of storage can be excluded from such treatment.

Suitable plants that can be treated in accordance with the present invention include dicots and monocots, including agricultural, silvicultural, ornamental and horticultural plants, whether in a natural or genetically modified form. Exemplary plants include, without limitation, alfalfa, apple, apricot, asparagus, avocados, bananas, barley, beans, beech (Fagus spec.), begonia, birch, blackberry, blueberry, cabbage, camphor, canola, carrot, castor oil plant, cherry, cinnamon, citrus, cocoa bean, coffee, corn, cotton, cucumber, cucurbit, eucalyptus, fir, flax, fodder beet, fuchsia, garlic, geranium, grapes, ground nut, hemp, hop, juneberry, juncea (Brassica juncea), jute, lentil, lettuce, linseed, melon, mustard, nectarine, oak, oats, oil palm, oil-seed rape, olive, onion, paprika, pea, peach, pear, pelargonium, peppers, petunia, pine (Pinus spec.), plum, poplar (Populus spec.), pome fruit, potato, rape, raspberry, rice, rubber tree, rye, sorghum, soybean, spinach, spruce, squash, strawberry, sugar beet, sugar cane, sunflower, tea, teak, tobacco, tomato, triticale, turf, watermelon, wheat and willow (Salix spec.), Arabidopsis thaliana, Saintpaulia, poinsettia, chrysanthemum, carnation, and zinnia.

With respect to modified biochemical signaling, this includes both enhancement of certain plant biochemical pathways and diminishment of certain other plant biochemical pathways. Biochemical signaling pathways that can be altered in accordance with the present invention include gene expression and protein production, production of metabolites, and production of signaling molecules/secondary metabolites. Exemplary biochemical signaling pathways and their modifications include, without limitation, induction of nitric oxide production, peroxide production, and other secondary metabolites; agonist of the ethylene signaling pathway and induction of ethylene-responsive gene expression (see Dong et al., Plant Phys. 136:3628-3638 (2004); Li et al., Planta 239:831-46 (2014); Chang et al., PLoS One 10, e0125498 (2015), each of which is hereby incorporated by reference in its entirety); agonist of the salicylic acid signaling pathway and induction of salicylic acid-responsive gene expression (see Dong et al., Plant J. 20:207-215 (1999), which is hereby incorporated by reference in its entirety); agonist of the abscisic acid pathway and induction of abscisic acid-responsive gene expression (see Dong et al., Planta 221: 313-327 (2005), which is hereby incorporated by reference in its entirety); agonist of the gibberellin signaling pathway and induction of gibberellin-responsive gene expression (see Li et al., Planta 239:831-46 (2014), which is hereby incorporated by reference in its entirety); antagonist of jasmonic acid signaling and inhibiting expression of jasmonic acid-responsive genes (see Dong et al., Plant Phys. 136:3628-3638 (2004), which is hereby incorporated by reference in its entirety); inducing protease inhibitor expression (see Laluk and Mengiste, Plant J. 68:480-494 (2011); Xia et al., Chin. Sci. Bull 56: 2351-2358 (2011), each of which is hereby incorporated by reference in its entirety); inducing reactive oxygen species production in plant tissues; inducing immune-related and antimicrobial peptide production, such as, without limitation, peroxidase, superoxide dismutase, chitinase, and β-1,3-glucanase (Wang et al., J. Agric. Food Chem. 59:12527-12533 (2011), which is hereby incorporated by reference in its entirety); and inducing expansin gene expression and production (see Li et al., Planta 239:831-46 (2014), which is hereby incorporated by reference in its entirety).

With respect to disease resistance, absolute immunity against infection may not be conferred, but the severity of the disease is reduced and symptom development is delayed. Lesion number, lesion size, and extent of sporulation of fungal pathogens are all decreased. This method of imparting disease resistance has the potential for treating previously untreatable diseases, treating diseases systemically which might not be treated separately due to cost, and avoiding the use of infectious agents or environmentally harmful materials.

The method of imparting pathogen resistance to plants in accordance with the present invention is useful in imparting resistance to a wide variety of pathogens including viruses, bacteria, and fungi. Resistance, inter alia, to the following viruses can be achieved by the method of the present invention: Tobacco mosaic virus and Tomato mosaic virus. Resistance, inter alia, to the following bacteria can also be imparted to plants in accordance with present invention: pathogenic Pseudomonas spp., pathogenic Erwinia spp., pathogenic Xanthomonas spp., and pathogenic Ralstonia spp. Plants can be made resistant, inter alia, to the following fungi by use of the method of the present invention: Fusarium spp. and Phytophthora spp.

With regard to the use of the recombinant host cell or compositions of the present invention to enhance plant growth, various forms of plant growth enhancement or promotion can be achieved. This can occur as early as when plant growth begins from seeds or later in the life of a plant. For example, plant growth according to the present invention encompasses greater yield, increased plant vigor, increased vigor of seedlings (i.e., post-germination), increased plant weight, increased biomass, increased number of flowers per plant, higher grain and/or fruit yield, increased quantity of seeds produced, increased percentage of seeds germinated, increased speed of germination, increased plant size, decreased plant height (for wheat), greater biomass, more and bigger fruit, earlier fruit coloration, earlier bud, fruit and plant maturation, more tillers or side shoots, larger leaves, delayed leaf senescence, increased shoot growth, increased root growth, altered root/shoot allocation, increased protein content, increased oil content, increased carbohydrate content, increased pigment content, increased chlorophyll content, increased total photosynthesis, increased photosynthesis efficiency, reduced respiration (lower O₂ usage), compensation for yield-reducing treatments, increased durability of stems (and resistance to stem lodging), increased durability of roots (and resistance to root lodging), better plant growth in low light conditions, and combinations thereof. As a result, the present invention provides significant economic benefit to growers. For example, early germination and early maturation permit crops to be grown in areas where short growing seasons would otherwise preclude their growth in that locale. Increased percentage of seed germination results in improved crop stands and more efficient seed use. Greater yield, increased size, and enhanced biomass production allow greater revenue generation from a given plot of land.

With regard to the use of the recombinant host cell or compositions of the present invention to control pests (including but not limited to insects and nematodes, which are biotic stressors), such pest control encompasses preventing pests from contacting plants to which the recombinant host cell or composition of the invention has been applied, preventing direct damage to plants by feeding injury, causing pests to depart from such plants, killing pests proximate to such plants, interfering with insect larval feeding on such plants, preventing pests from colonizing host plants, preventing colonizing insects from releasing phytotoxins, interfering with egg deposition on host plants, etc. The present invention also prevents subsequent disease damage to plants resulting from pest infection.

The present invention is effective against a wide variety of insects (biotic stressors). European corn borer is a major pest of corn (dent and sweet corn) but also feeds on over 200 plant species including green, wax, and lima beans and edible soybeans, peppers, potato, and tomato plus many weed species. Additional insect larval feeding pests which damage a wide variety of vegetable crops include the following: beet armyworm, cabbage looper, corn ear worm, fall armyworm, diamondback moth, cabbage root maggot, onion maggot, seed corn maggot, pickleworm (melonworm), pepper maggot, and tomato pinworm.

Collectively, this group of insect pests represents the most economically important group of pests for vegetable production worldwide. The present invention is also effective against nematodes, another class of economically important biotic stressors. Soybean Cyst Nematode (Heterodera glycines) is a major pest of soybeans. Reniform Nematode (Rotylenchulus reniformis) is a major pest of cotton as can parasitize additional crop species, notably soy and corn. Additional nematode pests include the root knot nematodes of the genus Meloidogyne (particularly in cotton, wheat, and barley), cereal cyst nematodes of the genus Heterodera (particularly in soy, wheat, and barley), root lesion nematodes of the genus Pratylenchus, seed gall nematodes of the genus Anguina (particularly in wheat, barley, and rye), and stem nematodes of the genus Ditylenchus. Other biotic stressors include arachnids, weeds, and combinations thereof.

With regard to the use of the recombinant host cells or compositions of the present invention to impart abiotic stress resistance to plants, such abiotic stress encompasses any environmental factor having an adverse effect on plant physiology and development. Examples of such environmental stress include climate-related stress (e.g., drought, flood, frost, cold temperature, high temperature, excessive light, and insufficient light), air pollution stress (e.g., carbon dioxide, carbon monoxide, sulfur dioxide, NOR, hydrocarbons, ozone, ultraviolet radiation, acidic rain), chemical (e.g., insecticides, fungicides, herbicides, heavy metals), nutritional stress (e.g., over- or under-abundance of fertilizer, micronutrients, macronutrients, particularly potassium, nitrogen derivatives, and phosphorus derivatives), and improved healing response to wounding. Use of recombinant host cells of the present invention imparts resistance to plants against such forms of environmental stress.

The methods of the present invention involving application of the recombinant host cell or composition can be carried out through a variety of procedures when all or part of the plant is treated, including leaves, stems, roots, propagules (e.g., cuttings), fruit, etc. Recombinant host cells can be applied in the form of an aqueous solution comprising a suspension of such beneficial microbes, which is then applied to the plant by spraying, coating, or immersion as described above. When treating plant seeds, in accordance with the application embodiment of the present invention, the microbes can be applied by low pressure spraying, coating, immersion (e.g., soaking), or injection. Other suitable application procedures can be envisioned by those skilled in the art provided they are able to effect contact of the beneficial microbes with cells of the plant or plant seed. In accordance with the application embodiment of the present invention, the beneficial microbes can be applied to plants or plant seeds in dry form. By way of example, dry application of microbes can be accomplished using bacterial or fungal products such as Kodiak® HB, available from Chemtura, and T-22™ HC, available from BioWorks. Once treated with the microbes of the present invention, the seeds can be planted in natural or artificial soil and cultivated using conventional procedures to produce plants. After plants have been propagated from seeds treated in accordance with the present invention, the plants may be treated with one or more applications of the microbes of the invention or compositions of the invention, to impart disease resistance to plants, to enhance plant growth, to control insects on the plants, to impart biotic or abiotic stress tolerance, to improve desiccation resistance of removed cuttings, to impart post-harvest disease resistance or desiccation resistance to harvested fruit or vegetables, and/or improved longevity of fruit or vegetable ripeness for harvested fruit or vegetables.

The recombinant host cells or compositions of the invention can be applied to plants or plant seeds in accordance with the present invention alone or in a mixture with other materials. Alternatively, the recombinant host cells or compositions can be applied separately to plants with other materials being applied at different times.

EXAMPLES

The following examples are provided to illustrate embodiments of the present invention but are by no means intended to limit its scope.

Example 1—Design of Peptide Expression Plasmids

Briefly, protein expression constructs were made incorporating one of the following harpin peptides: P5-21 (SEEQLELLLAFIAAALQQEE (SEQ ID NO: 4), which is also described in U.S. Provisional Patent Application Ser. No. 62/319,138 as SEQ ID NO: 33), P4-111 (SQGISEKQLDQLLSQLI (SEQ ID NO: 5), which is also described in U.S. patent application Ser. No. 15/244,919 as SEQ ID NO: 132), or P30-3 (LEELLEELIEELLEE (SEQ ID NO: 6), which is also described in U.S. patent application Ser. No. 14/872,298 as SEQ ID NO: 190). The expression construct further contained a fluorescent protein fusion for easy detection and increased stability in live cells along with a polyhistidine tag for easy purification. These expression constructs are identified in Table 1 below.

Red fluorescent protein sequences Fresno and Yukon were obtained from ATUM (Newark, Calif., USA). The pBE-S Bacillus subtilis expression plasmid was obtained from Clontech/Takara Bio USA (Mountain View, Calif., USA). The sequence of the pBE-S plasmid and the associated user manual are published at the following address: www.clontech.com/US/Products/Protein_Expression_and_Purification/Bacterial_Expression_Systems/High_Yield_Expression/B_subtilis_Secretory_Protein. These are hereby incorporated by reference.

The sequences for the above peptides were added to the C-terminus of the fluorescent protein sequence and were reverse-transcribed using a Bacillus subtilis codon bias table from the following address: www.kazusa.or.jp/codon/cgi-bin/showcodon.cgi?species=1423. These sequences were prepared for insertion into the Bacillus subtilis expression vector pBE-S by adding context sequence from the plasmid. This includes: 30 base pairs of plasmid sequence upstream of the MluI cleavage site in the pBE-S MCS and 30 base pairs of plasmid sequence downstream of the XbaI cleavage site. These DNA sequences were synthesized commercially as dsDNA, shown as SEQ ID NOs: 7-12 below.

The nucleic acid sequence of Fresno-P30-3 (SEQ ID NO: 7) is as follows:

TAAGTCTAGTCTGAACTTAAGCAAAAGGAGAGGGACGCGTATGAATTGAG TGATTAAAGAAAATATGCATATGAAACTGTATATGGAAGGCACAGTTAAT AATCATCATTTTAAATGCACATCAGAAGGCGAAGGCAAACCGTATGAAGG CACACAAACAATGAGAATTAAAGTTGTTGAAGGCGGCCCGCTGCCGTTTG CATTTGATATTCTGGCAACATCATTTATGTATGGCTCAAGAACATTTATT AAATATCCGAAAGGCATTCCGGATTTTTTTAAACAATCATTTCCGGAAGG CTTTACATGGGAAAGAGTTACAAGATATGAAGATGGCGGCGTTGTTACAG CAACACAAGATACATCACTGGAAGATGGCTGCCTGGTTTATCATGTTCAA GTTAGAGGCGTTAATTTTCCGTCAAATGGCCCGGTTATGCAAAAAAAAAC ACTGGGCTGGGAACCGAATACAGAAATGCTGTATCCGGCAGATGGCGGCC TGGAAGGCAGATCAGATATGGCACTGAAACTGGTTGGCGGCGGCCATCTG TCATGCTCATTTGTTACAACATATAGATCAAAAAAAACAGTTGGCAATAT TAAAATGCCGGGCATTCATGCAGTTGATCATAGACTGGTTAGAATTAAAG AAGCAGATAAAGAAACATATGTTGAACAACATGAAGTTGCAGTTGCAAAA TTTGCAGGCCTGGGCGGCGGCATGGATGAACTGTATAAATTAGAGGAACT GCTTGAAGAATTAATTGAAGAATTGCTCGAAGAGTCTAGACATCACCATC ATCACCACTAATGCGGTAGTTTAT

The nucleic acid sequence of Yukon-P30-3 (SEQ ID NO: 8) is as follows:

TAAGTCTACTCTGAACTTAAGCAAAAGGAGAGGGACGCGTATGTCTCTTT CCAAGCAGGTCCTTCCGCGTGATGTTCGTATGAGATTTCATATGGATGGG TGTGTTAATGGACATCAATTTACTATTGAAGGTGAAGGTGCTGGGAAACC GTATGAAGGTAAAAAAACATTGAAACTGAGAGTGACAAAAGGTGGGCCTC TTCCCTTCGCCTTCGATATACTTTCAGCAACATTTACGTATGGCAATCGG TGCTTTTGTGATTACCCGGAAGATATGCCGGACTATTTCAAACAAAGTTT GCCGGAGGGATACTCATGGGAACGAACGCTGATGTTTGAGGATGGGGGTT GCGGCACAGCGTCCGCGCACATTTCGTTAGAGAAAGACTGTTTCATTCAC AACAGCACTTTTCATGGGGTAAATTTCCCAGCAAACGGACCTGTAATGCA GAAAAAAACACTGAATTGGGAACCTTCATCCGAGCTGATTACGGCTTGTG ATGGCATCCTGAAGGGGGATGTCACAATGTTTTTACTGCTTGAGGGCGGA CACCGATTAAAGTGTCAATTCACAACGTCCTATAAGGCCCATAAGGCAGT GAAAATGCCGCCGAATCATATTATTGAACATGTGCTGGTAAAAAAAGAGG TCGCCGACGGTTTCCAGATTCAGGAACATGCCGTCGCAAAACATTTTACC GTGGATGTCAAGGAAACATTAGAGGAACTGCTTGAAGAATTAATTGAAGA ATTGCTCGAAGAGTCTAGACATCACCATCATCACCACTAATGCGGTAGTT TAT

The nucleic acid sequence of Fresno-P4-111 (SEQ ID NO: 9) is as follows:

TAAGTCTAGTCTGAACTTAAGCAAAAGGAGAGGGACGCGTATGAATTGAG TGATTAAAGAAAATATGCATATGAAACTGTATATGGAAGGCACAGTTAAT AATCATCATTTTAAATGCACATCAGAAGGCGAAGGCAAACCGTATGAAGG CACACAAACAATGAGAATTAAAGTTGTTGAAGGCGGCCCGCTGCCGTTTG CATTTGATATTCTGGCAACATCATTTATGTATGGCTCAAGAACATTTATT AAATATCCGAAAGGCATTCCGGATTTTTTTAAACAATCATTTCCGGAAGG CTTTACATGGGAAAGAGTTACAAGATATGAAGATGGCGGCGTTGTTACAG CAACACAAGATACATCACTGGAAGATGGCTGCCTGGTTTATCATGTTCAA GTTAGAGGCGTTAATTTTCCGTCAAATGGCCCGGTTATGCAAAAAAAAAC ACTGGGCTGGGAACCGAATACAGAAATGCTGTATCCGGCAGATGGCGGCC TGGAAGGCAGATCAGATATGGCACTGAAACTGGTTGGCGGCGGCCATCTG TCATGCTCATTTGTTACAACATATAGATCAAAAAAAACAGTTGGCAATAT TAAAATGCCGGGCATTCATGCAGTTGATCATAGACTGGTTAGAATTAAAG AAGCAGATAAAGAAACATATGTTGAACAACATGAAGTTGCAGTTGCAAAA TTTGCAGGCCTGGGCGGCGGCATGGATGAACTGTATAAATCGCAAGGAAT TAGTGAGAAACAGCTAGATCAACTATTATCTCAGCTCATATCTAGACATC ACCATCATCACCACTAATGCGGTAGTTTAT

The nucleic acid sequence of Yukon-P4-111 (SEQ ID NO: 10) is as follows:

TAAGTCTACTCTGAACTTAAGCAAAAGGAGAGGGACGCGTATGTCACTGT CAAAACAAGTTCTGCCGAGAGATGTTAGAATGAGATTTCATATGGATGGC TGCGTTAATGGCCATCAATTTACAATTGAAGGCGAAGGCGCAGGCAAACC GTATGAAGGCAAAAAAACACTGAAACTGAGAGTTACAAAAGGCGGCCCGC TGCCGTTTGCATTTGATATTCTGTCAGCAACATTTACATATGGCAATAGA TGCTTTTGCGATTATCCGGAAGATATGCCGGATTATTTTAAACAATCACT GCCGGAAGGCTATTCATGGGAAAGAACACTGATGTTTGAAGATGGCGGCT GCGGCACAGCATCAGCACATATTTGAGTGGAAAAAGATTGCTTTATTCAT AATTCAACATTTCATGGCGTTAATTTTCCGGCAAATGGCCCGGTTATGCA AAAAAAAACACTGAATTGGGAACCGTCATCAGAACTGATTACAGCATGCG ATGGCATTCTGAAAGGCGATGTTACAATGTTTCTGCTGCTGGAAGGCGGC CATAGACTGAAATGCCAATTTACAACATCATATAAAGCACATAAAGGAGT TAAAATGCCGCCGAATCATATTATTGAACATGTTCTGGTTAAAAAAGAAG TTGCAGATGGCTTTCAAATTCAAGAACATGCAGTTGCAAAACATTTTACA GTTGATGTTAAAGAAACATCGCAAGGAATTAGTGAGAAACAGCTAGATCA ACTATTATCTCAGCTGATATCTAGACATCACCATCATGAGCACTAATGCG GTAGTTTAT

The nucleic acid sequence of Fresno P5-21 (SEQ ID NO: 11) is as follows:

TAAGTCTACTCTGAACTTAAGCAAAAGGAGAGGGACGCGTATGAATAGTC TTATCAAAGAGAACATGCATATGAAACTGTATATGGAAGGGAGAGTGAAT AACCATCACTTCAAGTGTACCTCTGAAGGAGAAGGGAAACCGTATGAAGG CACGCAAACGATGCGCATTAAAGTCGTTGAAGGCGGACCCTTACCATTTG CCTTTGACATTCTGGCAACGAGCTTTATGTATGGAAGCCGGACTTTTATT AAATACCCAAAAGGCATTCCAGATTTCTTTAAACAAAGCTTCCCAGAAGG GTTTACATGGGAACGGGTCACAAGATATGAAGACGGCGGAGTCGTGACGG CAACACAAGATACGAGTCTGGAAGATGGCTGCTTGGTATATCATGTACAA GTCAGAGGAGTAAACTTTCCGTCTAACGGCCCGGTAATGCAGAAAAAGAC TTTAGGGTGGGAACCGAATACGGAGATGCTTTATCCTGCAGATGGGGGCT TAGAAGGACGCTCAGACATGGCGTTAAAATTGGTCGGCGGCGGCCATCTT TCCTGTTCTTTCGTGACCACCTATCGATCTAAGAAAACTGTGGGTAACAT CAAAATGCCAGGGATCCACGCTGTCGATCATCGTTTAGTAAGAATCAAAG AAGCGGACAAAGAAACGTACGTCGAACAGCATGAAGTGGCAGTTGCTAAA TTTGCAGGTTTAGGAGGCGGTATGGATGAGTTGTACAAGTCAGAGGAACA ACTTGAACTGTTATTAGCATTTATCGCAGCCGCCCTTCAACAAGAAGAAT CTAGACATCACCATCATCACCACTAATGCGGTAGTTTAT

The nucleic acid sequence of Yukon-P5-21 (SEQ ID NO: 12) is as follows:

TAAGTCTACTCTGAACTTAAGCAAAAGGAGAGGGACGCGTATGTCTCTTT CCAAGCAGGTCCTTCCGCGTGATGTTCGTATGAGATTTCATATGGATGGG TGTGTTAATGGACATCAATTTACTATTGAAGGTGAAGGTGCTGGGAAACC GTATGAAGGTAAAAAAACATTGAAACTGAGAGTGACAAAAGGTGGGCCTC TTCCCTTCGCCTTCGATATACTTTCAGCAACATTTACGTATGGCAATCGG TGCTTTTGTGATTACCCGGAAGATATGCCGGACTATTTCAAACAAAGTTT GCCGGAGGGATACTCATGGGAACGAACGCTGATGTTTGAGGATGGGGGTT GCGGCACAGCGTCCGCGCACATTTCGTTAGAGAAAGACTGTTTCATTCAC AACAGCACTTTTCATGGGGTAAATTTCCCAGCAAACGGACCTGTAATGCA GAAAAAAACACTGAATTGGGAACCTTCATCCGAGCTGATTACGGCTTGTG ATGGCATCCTGAAGGGGGATGTCACAATGTTTTTACTGCTTGAGGGCGGA CACCGATTAAAGTGTCAATTCACAACGTCCTATAAGGCCCATAAGGCAGT GAAAATGCCGCCGAATCATATTATTGAACATGTGCTGGTAAAAAAAGAGG TCGCCGACGGTTTCCAGATTCAGGAACATGCCGTCGCAAAACATTTTACC GTGGATGTCAAGGAAACATCAGAGGAACAACTTGAACTGTTATTAGCATT TATCGCAGCCGCCCTTCAACAAGAAGAATCTAGACATCACCATCATCACC ACTAATGCGGTAGTTTAT

Example 2—Assembly of Expression Plasmids

pBE-S plasmid DNA was double-digested using the restriction enzymes MluI and XbaI (from New England Biolabs, Ipswitch, Mass., USA) according to manufacturer instructions and purified on PCR cleanup columns (Qiagen USA, Germantown, Md., USA). The synthesized dsDNA inserts were inserted into the cut pBE-S plasmid using the Gibson Assembly Hifi 1-Step Kit (Synthetic Genomics, La Jolla, Calif., USA) according to manufacturer instructions. The resulting plasmid DNA libraries were transformed into DH5alpha E. coli cells and plated on LB agar supplemented with 100 ug/ml carbenicillin. Select colonies were grown in 10 ml LB broth with 100 ug/ml carbenecillin and plasmid DNA collected by Mini-Prep (Qiagen). The fidelity of the cloning was verified by sequencing of the insert. Satisfactory clones were obtained for all plasmids except Fresno-p30-3. The coding sequence for each of these included: the fluorescent marker protein with the bioactive peptide and a 6×His tag at the C-terminal end. Protein sequences are listed as SEQ ID NOs: 13-18 in Table 1 below

TABLE 1 Construct SEQ ID Name Sequence NO: Fresno-P5-21 MNSLIKENMHMKLYMEGTVNNHHFKCTSEGEGKPYEGTQTMRIKV 13 VEGGPLPFAFDILATSFMYGSRTFIKYPKGIPDFFKQSFPEGFTW ERVTRYEDGGVVTATQDTSLEDGCLVYHVQVRGVNFPSNGPVMQK KTLGWEPNTEMLYPADGGLEGRSDMALKLVGGGHLSCSFVTTYRS KKTVGNIKMPGIHAVDHRLVRIKEADKETYVEQHEVAVAKFAGLG GGMDELYKSEEQLELLLAFIAAALQQEESRHHHHHH Yukon-P5-21 MSLSKQVLPRDVRMRFHMDGCVNGHQFTIEGEGAGKPYEGKKTLK 14 LRVTKGGPLPFAFDILSATFTYGNRCFCDYPEDMPDYFKQSLPEG YSWERTLMFEDGGCGTASAHISLEKDCFIHNSTFHGVNFPANGPV MQKKTLNWEPSSELITACDGILKGDVTMFLLLEGGHRLKCQFTTS YKAHKAVKMPPNHIIEHVLVKKEVADGFQIQEHAVAKHFTVDVKE TSEEQLELLLAFIAAALQQEESRHHHHHH Fresno-P4-111 MNSLIKENMHMKLYMEGTVNNHHFKCTSEGEGKPYEGTQTMRIKV 15 VEGGPLPFAFDILATSFMYGSRTFIKYPKGIPDFFKQSFPEGFTW ERVTRYEDGGVVTATQDTSLEDGCLVYHVQVRGVNFPSNGPVMQK KTLGWEPNTEMLYPADGGLEGRSDMALKVGGGHLSCSFVTTYRSK KTVGNIKMPGIHAVDHRLVRIKEADKETYVEQHEVAVAKFAGLGG GMDELYKSQGISEKQLDQLLSQLISRHHHHHH Yukon-P4-111 MSLSKQVLPRDVRMRFHMDGCVNGHQFTIEGEGAGKPYEGKKTLK 16 LRVTKGGPLPFAFDILSATFTYGNRCFCDYPEDMPDYFKQSLPEG YSWERTLMFEDGGCGTASAHISLEKDCFIHNSTFHGVNFPANGPV MQKKTLNWEPSSELITACDGILKGDVTMFLLLEGGHRLKCQFTTS YKAHKAVKMPPNHIIEHVLVKKEVADGFQIQEHAVAKHFTVDVKE TSQGISEKQLDQLLSQLISRHHHHHH Fresno-P30-3 MNSLIKENMHMKLYMEGTVNNHHFKCTSEGEGKPYEGTQTMRIKV 17 VEGGPLPFAFDILATSFMYGSRTFIKYPKGIPDFFKQSFPEGFTW ERVTRYEDGGVVTATQDTSLEDGCLVYHVQVRGVNFPSNGPVMQK KTLGWEPNTEMLYPADGGLEGRSDMALKLVGGGHLSCSFVTTYRS KKTVGNIKMPGIHAVDHRLVRIKEADKETYVEQHEVAVAKFAGLG GGMDELYKLEELLEELIEELLEESRHHHHHH Yukon-P30-3 MSLSKQVLPRDVRMRFHMDGCVNGHQFTIEGEGAGKPYEGKKTLK 18 LRVTKGGPLPFAFDILSATFTYGNRCFCDYPEDMPDYFKQSLPEG YSWERTLMFEDGGCGTASAHISLEKDCFIHNSTFHGVNFPANGPV MQKKTLNWEPSSELITACDGILKGDVTMFLLLEGGHRLKCQFTTS YKAHKAVKMPPNHIIEHVLVKKEVADGFQIQEHAVAKHFTVDVKE TLEELLEELIEELLEESRHHHHHH

Example 3—Expression of Fluorescent Transgene

Plasmid DNA for Fresno-p4-111, Yukon-p4-111, Fresno-p5-21, Yukon-p5-21, and Yukon p30-3 were transformed into Bacillus subtilis strain RIK1275 as described by the manufacturer of the plasmid and plated on LB plates supplemented with 10 ug/ml Kanamycin. Colonies from this plate were tested for visual evidence of fluorescence using a green laser light source (˜532 nm) and an amber-colored filter. Fluorescent colonies were observed for Yukon-p4-111, Fresno-p5-21, Yukon-p5-21, and Yukon p30-3, indicating the production of the protein insert in the Bacillus subtilis cells.

Example 4—Confirmation of Soluble Protein in Bacterial Cell Lysates

Fluorescent colonies from Example 3 were inoculated into 5 ml cultures of LB medium supplemented with 10 ug/ml Kanamycin and grown for 2 days with 170 rpm shaking at 37° C. Cells were harvested by centrifugation (5000 g for 15 minutes at 4° C.). The culture was decanted away from the cell pellet. The cell pellets were resuspended in 1 ml each of Bugbuster Protein Extraction Reagent (EMD Millipore, Billerica, Mass., USA) supplemented with 200 ug/ml of lysozyme. Lysis was allowed to proceed for 20 minutes at room temperature (20° C.). The lysates were centrifuged at 20,000 g for 10 minutes at 4° C. to separate soluble from insoluble proteins. A reddish supernatant was observed for Fresno-p5-21, suggesting that the recombinant protein was soluble and well-expressed. For the other samples, no color was observed in the supernatant, though some fluorescence was observed in the lysate pellet.

Example 5—Ni-NTA Chromatography of Fresno-p5-21

The lysate supernatant from Example 4 containing Fresno-p5-21 was mixed with 0.5 ml of settled NiNTA resin (5-Prime, Hilden, Germany) and was mixed by gentle rotation for 2 hours at 4° C. The resin was then poured into a small gravity-fed chromatography column. Red color from the lysate supernatant adhered to the column, turning it a reddish-purple color. The column was washed with 5 column volumes of 50 mM sodium phosphate pH 7.4, 200 mM NaCl. The protein was then eluted with 250 mM imidazole+100 mM NaCl, pH 7.5. Upon elution, the red color was released from the column, generating a red eluate. The column reverted to its normal blue color. This indicates that the fluorescent protein could be purified by NiNTA chromatography. Since the bioactive peptide is between the fluorescent protein and the polyhistidine purification tag, it is inferred that the eluted protein includes the harpin peptide sequence.

Example 6—Hypersensitive Response Testing of Fresno-p5-21 Purified from B. subtilis

The production and purification procedure of Examples 4 and 5 were scaled up to 1 L to produce a quantity of protein appropriate for hypersensitive response elicitation in tobacco leaves.

Briefly, 1 L of LB culture media was supplemented with 10 ug/ml Kanamycin and cells were grown as in Example 3 for 2 days in a baffled flask. Cells were harvested at 6000 g for 20 minutes at 4° C. Culture supernatant was removed from the cells and the cells were resuspended in 20 ml of Bugbuster Protein Extraction Reagent supplemented with 50 ug/ml lysozyme. The sample was gently rocked at room temperature for 30 minutes and then frozen on liquid nitrogen and stored at −80° C.

The sample was thawed on ice and a 1/50 volume of 500 mM imidazole was added for a final concentration of 10 mM imidazole. 8 ml of the sample was mixed with 2 ml of settled Ni-NTA agarose resin (5-Prime) end-over-end for 2 hours at 4° C. The column was then settled for 20 minutes and allowed to flow by gravity. The flowthrough was collected. The resin was washed with 5 column volumes of 50 mM sodium phosphate, 15 mM imidazole, 200 mM NaCl. Finally, the protein was eluted with 250 mM imidazole, pH 7.5. The protein eluted from the resin was further desalted using centrifugal filtration columns (EMD Millipore, 10 kDa molecular weight cutoff), replacing the imidazole buffer with 10 mM sodium phosphate. A 1 ml sample of protein was generated. The protein concentration was quantified by UV/Vis spectroscopy using a Nanodrop 2000 (Thermo Fisher Scientific, Waltham, Mass., USA). The spectrum included peaks at 280 nm (A=0.084 for 1 cm path) and 555 nm (A=0.045 for 1 cm path). Based on a theoretical ε280=24360 1/(M*cm) and a molecular weight of 29283 Da, the protein concentration was about 100 ug/ml.

This protein solution was infused into tobacco leaves for a hypersensitive response test as previously described The protein solution caused lesions after 2 days at a 1× concentration and a 2× dilution typical of HR. This result indicates that the recombinant harpin peptide produced from Bacillus subtilis is biologically active in plants.

Example 7—Application of B. subtilis Expressing Fresno-p5-21 to Plants Via Foliar Spray

Harpin proteins and Bacillus subtilis have separately been shown to improve plant health when applied as a leaf spray. It is believed that a foliar application of Bacillus subtilis expressing Fresno-p5-21 will cause multiple beneficial effects. The recombinant Bacillus subtilis will be supplied as a liquid product of an industrial-scale bacterial fermentation at a concentration of at least 1×10⁸ CFU/mL. At this concentration, the solution will be sprayed directly onto the plant. (Higher concentration formulations can be sold as a concentrate which would be diluted by the end user prior to application.)

Ideally, the plants will be treated before the onset of disease symptoms during the early growth stage of life (3-6 leaves). The plants will not be watered for 4 hours after application and the application will not be carried out within 4 hours of rainfall. In addition, the application site will have a minimum of airflow to prevent significant drift of the sprayed liquid. The liquid will be sprayed directly onto plant leaves until the leaf surfaces are dripping.

Positive and negative controls include: foliar spray with water, foliar spray with an aqueous solution containing P5-21, and foliar spray with a comparable CFU/mL of Subtilex® NG (Bacillus subtilis biological inoculant) available from BASF.

The resulting plants will be evaluated for one or more of the following effects: enhanced growth (such as wet and dry root mass), nematode resistance, and drought resistance.

Example 8—Application of B. subtilis Expressing Fresno-p5-21 to Plants Via Root Drench

Bacillus subtilis is a soil-dwelling microbe and harpin peptide application has been shown to affect root morphology. It is believed a root drench application of Bacillus subtilis expressing Fresno-p5-21 will cause multiple beneficial effects. As in Example 7, above, the Bacillus subtilis expressing Fresno-p5-21 is industrially produced. For this application, a solution of at least 1×10⁹ CFU/mL will be used. Ideally, the solution will be applied at the time of seed planting or soon after germination. As above, the application will be carried out when the soil is dry and rain is not expected.

This solution will be applied directly to dry soil within 4 inches of the plant stem or the seed. Application will continue until the soil is saturated or the bacterial culture begins to run off.

Positive and negative controls include: root drench with water, root drench with an aqueous solution containing P5-21, and root drench with a comparable CFU/mL of Subtilex® NG (Bacillus subtilis biological inoculant) available from BASF.

The resulting plants will be evaluated for one or more of the following effects: enhanced growth (such as wet and dry root mass), nematode resistance, and drought resistance. A comparison of the results following foliar spray in Example 7 and root drench in Example 8 will identify the best treatment(s) for the plants.

Sequence Listing

Submitted with this application is a Sequence Listing in the form of an ASCII text (.txt) file, which is hereby incorporated by reference into the specification of the application. The ASCII text file (51 KB) was created on May 12, 2022 and has the file name 20220615_Sequence_Listing_ST25_147459_000375.

Having thus described the basic concept of the invention, it will be rather apparent to those skilled in the art that the foregoing detailed disclosure is intended to be presented by way of example only, and is not limiting. Various alterations, improvements, and modifications will occur and are intended to those skilled in the art, though not expressly stated herein. These alterations, improvements, and modifications are intended to be suggested hereby, and are within the spirit and scope of the invention. Additionally, the recited order of processing elements or sequences, or the use of numbers, letters, or other designations therefore, is not intended to limit the claimed processes to any order except as may be specified in the claims. Accordingly, the invention is limited only by the following claims and equivalents thereto. 

1. A recombinant host cell comprising a transgene that comprises a promoter-effective nucleic acid molecule operably coupled to a nucleic acid molecule that encodes a plant effector polypeptide, wherein the recombinant host cell is a microbe having an endogenous gene that imparts a first benefit to a plant grown in the presence of the recombinant microbe and the plant effector polypeptide imparts a second benefit to the plant grown in the present of the recombinant microbe, wherein said first benefit and said second benefit are distinct, and wherein the encoded plant effector polypeptide comprises the amino acid sequence of either: (i) L-X-X-L-L-L-X-(F/L)-(I/L)-X-X-X-L (SEQ ID NO: 34), wherein X at position 3 is optional and, when present, is selected from D, isoD, E, γ-glutamate, Q, N, S, and G; and each X at positions 2, 7, 10, 11, and 12 is independently selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G; or (ii) (Q/E)-(Q/E)-(L/I/V/F)-X-X-(L/I/V/F)-(L/I/V/F)-(L/I/V/F)-X-(L/I/V/F)-(L/I/V/F)-X-X-X-(L/I/V/F)-(D/G/Q/E)-(D/G/Q/E) (SEO ID NO: 35) wherein X at position 5 is optional and, when present, is selected from D, isoD, E, γ-glutamate, Q, N, S, and G, and each X at positions 4, 9, 12, 13, and 14 is independently selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G; or (iii) (L/I/V/F)-X-X-(L/I/V/F)-(L/I/V/F)-(L/I/V/F)-X-(L/I/V/F)-(L/I/V/F)-X-X-X-(L/I/V/F)-(D/G/Q/E)-(D/G/Q/E) (SEQ ID NO: 36) wherein X at position 3 is optional and, when present, is selected from D, isoD, E, γ-glutamate, Q, N, S, and G, and each X at positions 2, 7, 10, 11, and 12 is independently selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G; or (iv) (Q/E)-(Q/E)-(L/I/V/F)-X-X-(L/I/V/F)-(L/I/V/F)-(L/I/V/F)-X-(L/I/V/F)-(LI/V/F)-X-X-X-(L/I/V/F), (SEQ ID NO: 37) wherein X at position 5 is optional and, when present, is selected from D, isoD, E, γ-glutamate, Q, N, S, and G, and each X at positions 4, 9, 12, 13, and 14 is independently selected from M, A, D, isoD, E, γ-glutamate, Q, N, S, and G.
 2. The recombinant host cell according to claim 1, wherein the microbe is a bacterium.
 3. The recombinant host cell according to claim 2, wherein the bacterium is selected from the group of Pseudomonas, Sphingomonas, Bacillus, Streptomyces, Rhizobium, Frankia, and Azospirillum.
 4. The recombinant host cell according to claim 2, wherein the bacterium is selected from the group of Agrobacterium radiobacter, Azotobacter chroococcum, Burkholderia cepacia, Delfitia acidovorans, Paenobacillus macerans, Pantoea agglomerans, and Serratia entomophilia.
 5. The recombinant host cell according to claim 1, wherein the microbe is a fungus.
 6. The recombinant host cell according to claim 5, wherein the fungus is selected from the group of Rhodotorula, Aspergillus and Trichoderma.
 7. The recombinant host cell according to claim 1, wherein the transgene is stably integrated into the genome of the microbe.
 8. The recombinant host cell according to claim 1, wherein the transgene is present in an expression vector.
 9. The recombinant host cell according to claim 8, wherein the expression vector is a phage, plasmid, viral, or retroviral vector.
 10. The recombinant host cell according to claim 8, wherein the expression vector comprises an origin of replication operable in the recombinant host cell. 11-19. (canceled)
 20. The recombinant host cell according to claim 1, wherein the recombinant microbe is epiphytic or endophytic.
 21. (canceled)
 22. The recombinant host cell according to claim 1, wherein the first benefit comprises providing nutrition to a plant, producing plant hormone analogs that stimulate growth or reduce stress signaling, or competing with pathogenic organisms.
 23. The recombinant host cell according to claim 1, wherein the second benefit comprises disease resistance, growth enhancement, tolerance and resistance to biotic stressors, tolerance to abiotic stress, desiccation resistance for cuttings removed from ornamental plants, post-harvest disease resistance or desiccation resistance to fruit or vegetables harvested from plants, and/or improved longevity of fruit or vegetable ripeness for fruit or vegetables harvested from plants.
 24. A composition comprising a plurality of recombinant host cells according to claim
 1. 25. The composition according to claim 24, wherein the composition is in the form of a dry powder.
 26. (canceled)
 27. The composition according to claim 24, wherein the composition is in the form of an aqueous solution or suspension.
 28. (canceled)
 29. A mixture comprising one or more plant seeds and a composition according to claim
 24. 30. A method for treating plant seeds comprising: providing one or more plant seeds; and applying to the provided one or more plant seeds a recombinant host cell according to claim
 1. 31. The method according to claim 30, wherein said applying comprises either: mixing a dry powder comprises the recombinant host cells with the one or more plants seeds; or soaking or spraying the one or more plant seeds with an aqueous solution or suspension comprising the recombinant host cells.
 32. (canceled)
 33. A method for treating plants comprising: providing one or more plants; and applying to the provided one or more plants a recombinant host cell according to claim
 1. 34. The method according to claim 33, wherein said applying comprises either: spraying the one or more plants with an aqueous solution or suspension comprising the recombinant host cells; or dusting the one or more plants with a dry powder comprising the recombinant host cells.
 35. (canceled)
 36. A method for treating plants comprising: applying to a locus where plants are being grown or are expected to be grown a recombinant host cell according to claim 1; and growing one or more plants at the locus where the recombinant host cell is applied.
 37. The method according to claim 36, wherein the recombinant host cell is applied prior to planting seeds or one or more seedlings at the locus.
 38. The method according to claim 36, wherein the recombinant host cell is applied after planting seeds or one or more seedlings at the locus. 39-40. (canceled)
 41. The method according to claim 36, wherein the recombinant host cell is applied to the locus while plants are being grown at the locus.
 42. (canceled)
 43. A method of imparting disease resistance to plants comprising: applying an effective amount of a recombinant host cell according to claim 1 to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to impart disease resistance to the plant.
 44. The method according to claim 43, wherein the disease is a viral disease, a bacterial disease, or a fungal disease. 45-51. (canceled)
 52. A method of enhancing plant growth comprising: applying an effective amount of a recombinant host cell according to claim 1 to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to enhance plant growth.
 53. The method according to claim 52, wherein the enhanced growth comprises improved plant vigor, increased plant weight, increased biomass, increased number of flowers per plant, higher grain and/or fruit yield, more tillers or side shoots, larger leaves, increased shoot growth, increased protein content, increased oil content, increased starch content, increased pigment content, increased chlorophyll content, and combinations thereof. 54-60. (canceled)
 61. A method of increasing a plant's tolerance to biotic stress comprising: applying an effective amount of a recombinant host cell according to claim 1 to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to increase the plant's tolerance to biotic stress factors selected from the group consisting of insects, arachnids, nematodes, weeds, and combinations thereof. 62-68. (canceled)
 69. A method of increasing a plant's tolerance to abiotic stress comprising: applying an effective amount of a recombinant host cell according to claim 1 to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to increase the plant's tolerance to abiotic stress factors selected from the group consisting of salt stress, water stress, ozone stress, heavy metal stress, cold stress, heat stress, nutritional stress, and combinations thereof. 70-95. (canceled)
 96. A method of modulating plant biochemical signaling comprising: applying an effective amount of a recombinant host cell claim 1 to a plant or plant seed or the locus where the plant is growing or is expected to grow, wherein said applying is effective to modulate plant biochemical signaling.
 97. The method according to claim 96, where the plant biochemical signaling is selected from the group consisting of induction of nitric oxide production, peroxide production, or a secondary metabolite; agonistic modulation of the ethylene signaling pathway and induction of ethylene-responsive gene expression; agonistic modulation of the salicylic acid signaling pathway and induction of salicylic acid-responsive gene expression; agonistic modulation of the abscisic acid pathway and induction of abscisic acid-responsive gene expression; agonistic modulation of the gibberellin signaling pathway and induction of gibberellin-responsive gene expression; antagonistic modulation of jasmonic acid signaling and inhibiting expression of jasmonic acid-responsive genes; inducing protease inhibitor expression; inducing reactive oxygen species production in plant tissues; inducing immune-related and antimicrobial peptide production; and inducing expansin gene expression and production.
 98. A recombinant host cell comprising a transgene that comprises a promoter-effective nucleic acid molecule operably coupled to a nucleic acid molecule that encodes a plant effector polypeptide, wherein the recombinant host cell is a microbe having an endogenous gene that imparts a first benefit to a plant grown in the presence of the recombinant microbe and the plant effector polypeptide imparts a second benefit to the plant grown in the present of the recombinant microbe, wherein said first benefit and said second benefit are distinct, and wherein the encoded plant effector polypeptide has the amino acid sequence consisting essentially of: Peptide Peptide Amino Sequence Name Acid Sequence Identifier P5 SAGSEQQLDLLLMFIMMMLQQ (SEQ ID NO: 38) P5a SAGSEQQLDQLLLMFIMMMLQQ (SEQ ID NO: 39) P5-21 SEEQLELLLAFIAAALQQEE (SEQ ID NO: 40) P5-25 SEEEEQLDQLLLAFIAAALQQ (SEQ ID NO: 41) P5-2 SAGSEQQLDLLLMFIAAALQQ (SEQ ID NO: 50) P5-3 SAGSEQQLDLLLAFIAAALQQ (SEQ ID NO: 51) P5-4 SAGSEQQLELLLAFIAAALQQ (SEQ ID NO: 52) P5-5 QLELLLAFIAAALQQ (SEQ ID NO: 53) P5-8 SEEEEELDLLLAFIAAALQQ (SEQ ID NO: 54) P5-14 SEEEEELDLLLAFIAAALGG (SEQ ID NO: 55) P5-19 SELELLLAFIAAALEEEEE (SEQ ID NO: 56) P5-23 SEEEEELDQLLLAFIAAALQQ (SEQ ID NO: 57) P5-26 SEEQLDLLLAFIAAALQEE (SEQ ID NO: 58) P5-28 SEEQLDQLLLAFIAAALEE (SEQ ID NO: 59) P5-29 SEEELDLLLMFIMMMLEE (SEQ ID NO: 60) P5-30 SEEELDQLLLMFIMMMLEE (SEQ ID NO: 61) P5-31 SEEEQLDLLLMFIMMMLEE (SEQ ID NO: 62) P5-32 SEEEQLDQLLLMFIMMMLEE (SEQ ID NO: 63) P5-33 SEEEQLDLLLMFIMMMLQEE (SEQ ID NO: 64) P5-34 SEEEQLDQLLLMFIMMMLQEE (SEQ ID NO: 65) P5-35 SAGSEQQEDLLLMFIMMMLQQ (SEQ ID NO: 66) P5-36 SAGSEQQLDELLMFIMMMLQQ (SEQ ID NO: 67). 